Compositions and methods for treating, preventing and/or reversing type-1 diabetes

ABSTRACT

The present invention relates generally compounds, compositions, combinations, kits, and methods for treatment; prevention, suppression, and/or delaying the onset of type 1 diabetes, or reversal of type 1 diabetes.

This application is a continuation-in-part of U.S. patent application Ser. No. 11/290,070, filed Nov. 9, 2005, which is a continuation-in-part of U.S. patent application Ser. No. 10/681,788, filed Oct. 8, 2003, which is a continuation-in-part of International Patent Application No. PCT/US03/10700, filed Apr. 8, 2003, which claims priority to U.S. Provisional Patent Application Ser. No. 60/371,663, filed Apr. 9, 2002; each of these applications are hereby incorporated by reference herein in their entirety.

This invention was made with Government support under NIH grant DK65748, awarded by the PHS. The Government has certain rights in the invention.

FIELD OF THE INVENTION

The present invention relates generally to methods, compounds and compositions useful for, inter alia, treating, preventing, suppressing or delaying the onset of, or reducing the risk of developing, type 1 diabetes, or reversing type 1 diabetes, or the symptoms associated with or related to type 1 diabetes.

BACKGROUND OF THE INVENTION

Type 1 diabetes, also known as insulin-dependent diabetes mellitus (“IDDM”), is an autoimmune disease in which the beta (“β”) cells of the pancreatic islets of Langerhans are destroyed as a consequence of inflammatory reactions triggered by activation of T cells specific for β-cell associated antigens (1, 2; see “Reference” section at the end of document). Data obtained from preclinical animal models of IDDM as well as clinical studies have implicated CD4⁺ and CD8⁺ autoreactive T cells as key effectors of islet cell destruction (J. F. Bach, Endocr. Rev., 1994). Despite the availability of insulin replacement therapy to maintain acceptable control of blood glucose levels, chronic insulin replacement therapy is still associated with major side effects including potential for acute hypoglycemia, chronic microvascular disease (retinopathy, nephropathy and neuropathy) and chronic macrovascular disease (heart disease and stroke) all resulting from the poor fine control of carbohydrate metabolism that can be attained with bolus injection of insulin (Simone et al., Diabetes Care, 22 Suppl. 2.: B7-B15, 1999). These side effects, combined with high cost, the invasive nature of insulin therapy and the increasing prevalence of IDDM in the developed world, have led to efforts for finding alternative strategies including methods of preventing progression from the inciting autoreactive process to the irreversible loss of over 90% of the islet mass that correlates with clinical presentation of disease.

The non-obese diabetic (“NOD”) mouse develops a spontaneous type 1 diabetes that shares many of the features associated with human IDDM providing a well characterized animal model for this complex autoimmune disease (3). The initial or pre-insulitis stage of disease begins around 3 weeks of age and involves cell infiltration in areas surrounding the pancreatic islets without damage of the β cells (4). The next phase of disease, known as insulitis, begins around the age of 6 weeks and involves a gradual increase in cell infiltration which ultimately overcomes the immunoregulatory mechanisms in place leading to a progressive destruction of the β cells (5). Complete loss of insulin production leads to dysregulation of glucose metabolism and overt diabetes can manifest as early as 12 weeks of age (6). It is now well accepted that progression from insulitis to diabetes correlates with a rise of Th1 type cells specific for β-cell associated antigens (7). Cytokines such as IFNγ and TNFα produced by these Th1 cells stimulate recruitment of inflammatory cells capable of β cell destruction (8-10). Hence, down-regulation of the Th1 cells would be a logical approach to combat diabetes. A number of antigen-specific strategies are being considered for modulation of the autoreactive T cells in NOD mice (11-14) as well as other animal models of IDDM (15, 16). The translation to human, however, is not yet in place and issues such as practicality, side effects, and efficacy have to be overcome in order for the transition to occur.

Recently, it has been shown that delivery of class II-restricted peptides on immunoglobulins (“Igs”) increases presentation to T cells by 100-fold relative to free peptide (17, 18). This is due to internalization of Igs via Fcγ receptors (“FcγR”) processing within the endosomal compartment and unlimited access of the peptides to newly synthesized MHC molecules (19). Given the fact that Igs are self-molecules, side effects are minimal even when repetitive injections are required. Furthermore, due to their autologous nature, when injected into animals without adjuvant, Igs do not induce inflammatory signals that up-regulate costimulatory molecules on antigen presenting cells (“APCs”) (20). Indeed, adjuvant-free regimens that used Igs to deliver antigenic peptides have proven effective for induction of tolerance rather than immunity (20-23). For instance, when PLP1 peptide, corresponding to the encephalitogenic sequence 139-151 of proteolipid protein (“PLP”), was expressed on an Ig molecule, the resulting Ig-PLP1 displayed modulatory functions against experimental allergic encephalomyelitis (“EAE”) and suppressed paralytic relapses (20, 22). Furthermore, aggregation of Ig-PLP1 led to cross-linking of FcγR and induction of IL-10 production by the presenting APCs (20, 22). Consequently, aggregated (“agg”) Ig-PLP1 displayed a greater potency against EAE inducing full and expeditious recovery from disease suppressing both the initial severe paralytic phase and the relapses (22). Neutralization of IL-10 by injection of anti-IL-10 antibody reversed the course of action of agg Ig-PLP1 and the disease rebounded indicating that endogenous IL-10 plays a critical role in the prevention of autoimmunity. Moreover, the Ig delivery approach proved effective with a myelin oligodendrocyte glycoprotein (“MOG”) peptide and Ig-MOG was able to suppress EAE even when disease induction used central nervous system (“CNS”) homogenate which includes multiple epitopes (23). The conclusion that has been drawn from these observations demonstrates that agg Ig chimeras couple endogenous IL-10 to peripheral tolerance setting into motion a multi-modal approach effective against complex autoimmunity involving diverse T cell specificities (20, 22, 23). In the NOD system, IL-10 has been shown to display variable effects on diabetes depending upon the mode of delivery (24-26) and the age of the animal (27-29). Apart from this variable function, the lack of a practical delivery strategy and the ill-defined mechanism underlying the mode of action of IL-10 justifies the search for new approaches to direct endogenous IL-10 against diverse diabetogenic T cells and prevent spontaneous diabetes in the NOD mouse.

Therefore, there is a need for additional treatment regimes for the treatment, prevention, and/or reduction in the risk of developing type 1 diabetes, or the symptoms associated with, or related to, type 1 diabetes, in a subject in need thereof.

SUMMARY OF THE INVENTION

In various embodiments, the present invention is directed to methods, compounds and compositions for treating, preventing, suppressing and/or delaying the onset, or reducing the risk of developing type 1 diabetes, or the symptoms associated with, or related to, type 1 diabetes, in a subject in need thereof. In other embodiments, the present invention is directed to methods for regenerating islet cells and/or to methods for reversing type 1 diabetes in a subject in need thereof,

In one embodiment, the present invention is directed to compounds, compositions, and methods for endocytic presentation of an immunosuppressive factor for the down regulation of diabetogenic T cells for the treatment or prevention of type 1 diabetes. In another embodiment, the invention relates to methods for slowing the onset of, or reversing or stopping the onset of, type-I diabetes that has progressed to the prediabetic stage. In another embodiment, compositions comprising at least one immunoglobulin, for example, INS, GAD, an insulin protein, a peptide derived from insulin, a diabetogenic epitope, or a T cell receptor engaging determinant, are provided to treat, prevent, suppress, or delay the onset of type 1 diabetes, for example after expression of an IAA predisposition marker.

The present invention also provides a method for the treatment or prevention of type 1 diabetes (or symptoms associated therewith) in a subject in need thereof. In one embodiment, the treatment or prevention is initiated during the pre-insulitis stage. In another embodiment, the treatment or prevention is initiated during the prediabetic stage. In yet another embodiment, the subject has not yet undergone IAA seroconversion when treatment is initiated. In still another embodiment, the treatment or prevention is initiated before and/or after the expression of one or more predisposition markers. In yet another embodiment, the subject may or may not have progressed to a hyperglycemic stage when treatment is initiated. In still another embodiment, treatment is initiated after the subject has been diagnosed with diabetes. The above methods comprise, inter alia, administering to a subject a composition that comprises an immunoglobulin, or portion thereof, linked to a peptide wherein the immunoglobulin or portion thereof is solubilized or aggregated.

In another embodiment, methods, compounds, and compositions of the present invention are directed to treating, preventing or reducing the risk of developing type 1 diabetes in an at-risk patient expressing a predisposition marker for type 1 diabetes.

In yet another embodiment, the present invention provides methods for preventing, delaying or reversing type 1 diabetes in a subject that is in the pre-diabetic stage. In one embodiment, a subject that is in the “pre-diabetic stage” herein is a subject that exhibits antibody positivity (presence of islet cell antibodies) and abnormal first phase insulin test (insulin response to an i.v. glucose bolus). In another embodiment, the present invention provides methods for preventing, delaying or reversing type 1 diabetes in a subject that has impaired glucose tolerance as defined herein below.

In yet another embodiment, the present invention provides methods for reversing diabetes in a subject in need thereof. In one embodiment, this method comprises the steps of: (a) diagnosing a subject as having diabetes, and (b) administering a composition as described herein to the subject.

In yet another embodiment, the present invention provides methods for regenerating islet cells in a subject in need thereof. In one embodiment, such a method comprises the steps of: (a) diagnosing a subject as having diabetes, and (b) administering a composition as described herein to the subject.

In another embodiment, the present invention also provides a composition comprising an immunoglobulin, or portion thereof, linked to a protein fragment or peptide wherein the immunoglobulin, or portion thereof, is capable of binding to an Fc receptor. In one embodiment, the peptide is derived from INS and/or GAD, such as, for example, INSβ, GAD 1 and GAD2. In yet another embodiment, the composition is capable of being endocytosed by cells bearing the Fc receptor and processed and presented by the cells to present the peptide to endogenous MHC Class II molecules, thereby substantially reducing or preventing activation of diabetogenic T cells specific for the peptide.

A method for presenting T cell receptor engaging determinant or epitope on the surface of a professional or nonprofessional antigen presenting cell is also provided by the present invention.

These and other embodiments of the invention will be described in more detail herein below.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows the nucleotide and amino acid sequences of the INSβ and HEL inserts as well as the flanking regions surrounding them within the heavy chain CDR3 of the 91A3 Ig. The lower panel of FIG. 1 shows secreted chimeric Ig in the supernatant from transfectoma cells indicating that complete constructs were created.

FIG. 2 demonstrates that the INSβ-specific T cell line proliferated significantly upon incubation with irradiated NOD splenic APCs and INSβ peptide (FIG. 2(a)), or Ig-INSβ (FIG. 2(b)), indicating that Ig-INSβ is taken up by the APCs and an INSβ peptide is generated and presented to T cells. FIGS. 2(c) and 2(d) indicate that presentation of INSβ and Ig-INSβ is specific.

FIG. 3 shows that insulin-specific autoantibodies can serve as a marker for early development of diabetes.

FIG. 4 shows dose dependent suppression of diabetes by soluble Ig-INSβ in IAA-positive NOD mice.

FIG. 5 shows that IL-10 secreted by APCs during presentation of agg Ig-INSβ antagonizes the production of IFNγ by INSβ-specific T cells.

FIG. 6 shows that agg Ig-INSβ reduces Th1 responses but supports production of IL-10 and TGFβ upon administration into NOD mice.

FIG. 7 shows that agg Ig-INSβ displays no significant delay of diabetes in IAA-positive mice.

FIG. 8 shows that the soluble form of Ig-INSβ is much more effective than the aggregated form in the suppression of diabetes.

FIG. 9 shows that treatment with agg Ig-INSβ at the pre-insulitis stage leads to effective suppression of diabetes.

FIG. 10 shows that administration of agg Ig-INSβ into IL-10^(−/−) NOD mice at the pre-insulitis stage does not delay onset of diabetes.

FIG. 11 illustrates that splenic and islet-infiltrating INSβ-specific T cells mount differential IFNγ responses upon stimulation with agg Ig-INSβ.

FIG. 12 shows that sustained administration of soluble Ig-INSβ to NOD mice after IAA seroconversion delays the onset of diabetes.

FIG. 13 A shows protection from diabetes in NOD mice when the mice were treated with sol Ig-GAD2 initiated at the hyperglycemic stage and continued for 15 or 25 weeks. 60% of mice under the 15 week regimen were protected from diabetes throughout the 25 week monitoring period. When the regimen was extended to 25 weeks, 100% of the mice were protected from diabetes.

FIG. 13 B shows that one mouse (open stars) progressed to diabetes by 5 weeks of treatment and 3 mice (plus, open diamond, open pentagon) had similar disease manifestations shortly after interruption of treatment.

FIG. 14 shows results of histopathologic analysis of mice treated with Ig-GAD2. Treated mice had a significantly greater number of islets when compared to both hyperglycemic and diabetic mice

FIG. 15 shows histopathologic slides of treated mice. Most islets in the treated mice were not inflamed (slide 4) or had only mild peri-insulitis (slides 5 and 6).

FIG. 16 shows analysis of islet infiltration scores among the different groups of mice. The 15-week group had a higher number of islets with per-insulitis (38% v. 30%) or no insulitis (35% v. 17%) relative to the hyperglycemic state. The number of islets with severe- and mild-intrainsulitis were reduced in the treated versus hyperglycemic mice (8% and 19% v. 22% and 31%, respectively. In the 25-week treatment group, although the total number of islets was reduced to that of the hyperglycemic stage, most of those islets exhibited no (60%), peri-(28%) or mild intra (12%) insulitis.

FIG. 17 shows a intestinal section from a mouse injected with the proliferation indicator 5-bromo-2-deoxyuridine (BRdU), sacrificed and stained with anti-insulin and anti-BrdU antibodies and analyzed for BrdU incorporation and insulin production. BrdU staining was visible in the highly proliferative luminal intestinal cells but these had no staining with anti-insulin antibody.

FIG. 18 shows that islets of non-diabetic 5-week old NOD mice were positive when stained with anti-insulin antibody, but did not incorporate BrdU, suggesting that these insulin-producing beta cells were not newly generated cells.

FIG. 19 shows the number of cells incorporating BrdU and/or producing insulin. Under normal circumstances, insulin production emanates from existing beta cells whose nuclei do not incorporate BrdU giving a minimal number of BrdU/insulin double-positive beta cells.

FIG. 20 shows sections from hyperglycemic mice that show very few insulin-producing beta cells and no BrdU incorporation resulting in an insignificant number of BrdU⁺/insulin⁺ beta cells.

FIG. 21 shows islets from the 25-week treatment group showing beta cells stained positive for insulin and were either BrdU negative (previously generated beta cells) or BrdU positive (newly generated beta cells). The number of insulin-producing regenerating beta cells was significantly increased in all five mice in which treatment restored normoglycemia.

DETAILED DESCRIPTION OF THE INVENTION

While the present invention is capable of being embodied in various forms, the description below of several embodiments is made with the understanding that the present disclosure is to be considered as an exemplification of the invention, and is not intended to limit the invention to the specific embodiments illustrated. For example, where the invention is illustrated herein with particular reference to Ig-INSβ, it will be understood that any other. immunoglobulin, such as Ig-CAD-1 or Ig-CAD2 can, if desired, be substituted in whole or in part for the Ig-INSβ in any embodiment of the invention. Headings are provided for convenience only and are not to be construed to limit the invention in any way. Embodiments illustrated under any heading may be combined with embodiments illustrated under any other heading.

The use of numerical values in the various ranges specified in this application, unless expressly indicated otherwise, are stated as approximations as though the minimum and maximum values within the stated ranges were both preceded by the word “about.” In this manner, slight variations above and below the stated ranges can be used to achieve substantially the same results as values within the ranges. As used herein, the terms “about” and “approximately” when referring to a numerical value shall have their plain and ordinary meanings to one skilled in the art of pharmaceutical sciences or the art relevant to the range or element at issue. The amount of broadening from the strict numerical boundary depends upon many factors. For example, some of the factors to be considered may include the criticality of the element and/or the effect a given amount of variation will have on the performance of the claimed subject matter, as well as other considerations known to those of skill in the art. Thus, as a general matter, “about” or “approximately” broaden the numerical value. For example, in some cases, “about” or “approximately” may mean ±5%, or ±10%, or ±20%, or ±30% depending on the relevant technology. Also, the disclosure of ranges is intended as a continuous range including every value between the minimum and maximum values.

It is also to be understood that any ranges, ratios and ranges of ratios that can be formed by any of the numbers or data present herein represent further embodiments of the present invention. This includes ranges that can be formed that do or do not include a finite upper and/or lower boundary. Accordingly, the skilled person will appreciate that many such ratios, ranges, and ranges of ratios can be unambiguously derived from the data and numbers presented herein and all represent embodiments of the present invention.

The present invention is directed to methods, kits, combinations, and compositions for treating, preventing, suppressing, delaying or reversing the onset of a disease, condition or disorder where treatment with an anti-diabetic type 1 agent is indicated.

In one embodiment of the present invention, the immunosuppressive factor for the down regulation of diabetogenic T cells comprises an immunoglobulin, or a portion thereof, linked to a protein fragment or peptide. In yet another embodiment, the immunoglobulin, or portion thereof, can bind, or is capable of binding, to an Fc receptor. The present invention is also directed to methods, kits, combinations, and compositions comprising a pharmaceutically-effective amount of a composition comprising an immunoglobulin, or a portion thereof, linked to a peptide, wherein the immunoglobulin or portion thereof is soluble or aggregated.

The present invention is also directed to a methods, kits, combinations, and compositions, comprising: a pharmaceutically-effective amount of an immunoglobulin, or portion thereof, linked to a protein fragment or peptide, wherein the immunoglobulin, or portion thereof, can bind to an Fc receptor. Illustratively, such a peptide comprises INSβ, GAD 1, or GAD2. In an additional embodiment, the composition is capable of being endocytosed by cells comprising the Fc receptor and processed by the cells to present the peptide to endogenous MHC Class II molecules, thereby substantially reducing or preventing activation of diabetogenic T cells specific for the peptide. In one embodiment, the peptide is inserted within a variable region of the immunoglobulin, or portion thereof.

The present invention is also directed to a use of a composition for the preparation of a pharmaceutical composition for alleviating symptoms associated with type 1 diabetes in a subject in need thereof, wherein the composition comprises a pharmaceutically-effective amount of an immunoglobulin, or portion thereof, linked to one or more peptides. In a related embodiment, the immunoglobulin, or portion thereof, can bind to an Fc receptor and be endocytosed by an antigen presenting cell, and the one or more peptides, or fragments thereof, provide one or more T cell receptor engaging determinants for presentation on the surface of the antigen presenting cell upon endocytic processing.

The present invention also provides a method for presenting a T cell receptor engaging determinant on the surface of a professional or nonprofessional antigen presenting cell, comprising: a) providing a composition comprising an immunoglobulin, or portion thereof, linked to one or more peptides derived from the group consisting of insulin and GAD. The immunoglobulin, or portion thereof, can bind to an Fc receptor and be endocytosed by an antigen presenting cell, and the one or more peptides, or fragments thereof, provide one or more T cell receptor engaging determinants for presentation on the surface of the antigen presenting cell upon endocytic processing; b) contacting the composition with at least one Fc receptor present on a surface of a professional or nonprofessional antigen presenting cell, wherein the composition is internalized by the antigen presenting cell; and c) endocytically processing the internalized composition to provide one or more T cell receptor engaging determinants; wherein the provided T cell receptor engaging determinants are presented on the surface of the antigen presenting cell.

In one embodiment, the T cell receptor engaging determinant is presented on the surface of the antigen presenting cells associated with at least on MHC complex.

Besides being useful for human treatment, the present invention is also useful for other subjects including veterinary animals, reptiles, birds, exotic animals and farm animals, including mammals, rodents, and the like. Mammals include horses, dogs, pigs, cats or primates, for example, a monkey, chimpanzee or a lemur. Rodents include rats, mice, squirrels, or guinea pigs.

In one embodiment of the present invention, methods, kits, combinations, and compositions containing at least one immunoglobulin, for example, INS, GAD, an insulin protein, a peptide derived from insulin, a diabetogenic epitope, or a T cell receptor engaging determinant, are provided to treat, prevent, suppress, reverse or delay the onset of type 1 diabetes after expression of an IAA predisposition marker. In yet another embodiment, IL-10 is substantially not required for the treatment, prevention, suppression, or delay in the onset of type 1 diabetes.

In one embodiment, a method of treating, preventing, suppressing, reversing or delaying the onset of type 1 diabetes during the pre-insulitis stage of diabetes is provided. The method comprises administering to a subject a pharmaceutically-effective amount of a composition comprising an immunoglobulin, or a portion thereof, linked to a peptide, wherein the immunoglobulin, or a portion thereof, is aggregated or solublized.

In another embodiment, the present invention provides a method of delaying, preventing, treating or reversing the onset of type 1 diabetes in a subject while or after the subject has reached the pre-diabetic stage or while the subject has impaired glucose tolerance. The method comprises administering to a subject a pharmaceutically-effective amount of a composition of the invention while the subject is in the pre-diabetic stage as defined above, or while the subject exhibits impaired glucose tolerance.

In yet another embodiment of the present invention, the aggregated immunoglobulin, or a portion thereof, can bind, or is capable of binding, to an Fc receptor and the peptide is presented to T cells in association with MHC class II molecules.

In one embodiment of the present invention, the compound is administered to the subject in the preinsultis stage of type 1 diabetes. In yet another embodiment of the present invention, the compound is administered to the subject before the subject has undergone IAA seroconversion. In yet another embodiment of the present invention, the compound is administered to the subject before the subject has seroconverted and produces autoantibodies against one or more β-cell associated antigens. In still another embodiment of the present invention, the compound administered to a subject that is IAA-positive. In yet another embodiment, the compound is administered to a subject before the subject has developed hyperglycemia. In another embodiment of the invention, the subject has developed hyperglycemia when treatment is initiated.

The present invention is also directed to a method of treating, preventing, or delaying the onset of type 1 diabetes, in a subject expressing a type 1 diabetes predisposition marker.

In another embodiment of the present invention, the aggregated immunoglobulin, or portion thereof, can bind to, or is capable of binding to, an Fc receptor. In one embodiment, the Fc receptor is an Fcγ receptor.

In yet another embodiment, the peptide is presented to T cells in association with MHC class II molecules. In one embodiment, the peptide is an INSβ peptide.

In another embodiment, compositions of the invention are capable of being endocytosed by cells having an Fe receptor and are processed and presented by the cells in association with MHC class II molecules thereby substantially reducing or preventing activation of diabetogenic T cells.

In yet another embodiment, administration of the composition of the present invention to a subject predisposed for type 1 diabetes delays the onset of type 1 diabetes. In another embodiment, the administration of the composition of the present invention to a subject induces production of IL-10.

In yet another embodiment of the present invention, the immunoglobulin comprises Ig-INSβ, Ig-GAD1, Ig-GAD2, or an immunoglobulin, or a portion thereof, linked to a peptide, for example a peptide derived from GAD65 or an insulin protein. In another embodiment of the present invention, the immunoglobulin, or a portion thereof, has more than one peptide linked to the immunoglobulin. In yet another embodiment, the immunoglobulin is solubilized, for example, solubilized Ig-INSβ, solubilized Ig-GAD1, or solubilized Ig-GAD2. In yet another embodiment of the present invention, the immunoglobulin is aggregated. In still another embodiment of the present invention, the immunoglobulin, or a portion thereof, can be human or humanized, such as, for example, human IgG, such as IgG1, IgG2, IgG2a, IgG2b, IgG3 and/or IgG4.

In yet another embodiment, the T cells are specific for the peptide. In another embodiment, the peptide is a T cell receptor engaging determinant. In yet another embodiment, the peptide comprises a diabetogenic epitope. In still another embodiment, the peptide is a INSβ peptide. In still another embodiment of the present invention, the peptide is derived from insulin.

In one embodiment, the peptide is inserted within the variable region of the immunoglobulin, or a portion thereof, and the immunoglobulin, or a portion thereof, comprises human IgG or humanized IgG.

In still another embodiment, the peptide is inserted within at least one of the variable regions of the immunoglobulin, or a portion thereof, comprising the CDR1, CDR2, and/or CDR3 region. Illustratively, the peptide is inserted within the CDR3 region of the immunoglobulin, or a portion thereof, by deleting the D segment and insertion of the peptide.

In one embodiment, the peptide comprises GAD1 and/or GAD2. In yet another embodiment, the composition comprises IgINS (peptides derived from human insulin), IgGAD (peptides derived from GAD), IgINSβ, IgGAD1 and IgGAD2.

In yet another embodiment, the invention provides a method of treatment of type 1 diabetes in an at-risk subject expressing a predisposition marker for type 1 diabetes. The method comprises administering to the subject a composition comprising an immunoglobulin or portion thereof linked to a diabetogenic peptide, optionally wherein the composition is soluble. In another embodiment, the subject is in the pre-insulitis stage of type 1 diabetes, or expresses a predisposition marker (IAA positive and/or GAD positive), or expresses a predisposition marker but has not yet progressed to a hyperglycemic stage. In another embodiment, the subject has been diagnosed with diabetes.

In another embodiment, the present invention provides a composition that enhances IL-10 production in splenic T cells. In still another embodiment, the composition induces production of IL-10 and/or induces production of IL-10 by APCs thereby enhancing peripheral tolerance to the onset of diabetes at the pre-insulitis stage. In another embodiment, a composition of the present invention induces production of TGFβ and/or IL-10 producing cells. In yet another embodiment, the composition, when administered to a subject, delays the onset of type 1 diabetes. In still another embodiment, the subject is at the pre-insulitis stage, following seroconversion, and/or at the pre-diabetic stage.

In one embodiment of the present invention, the T cells are nonproliferative antigen specific T cells. In another embodiment of the present invention, the aggregated Ig-INSβ compositions cross-link Fcγ receptors.

In one embodiment of the present invention, the composition is administered daily (or 1 to 5 times daily), weekly, or monthly. Illustratively, the composition is administered weekly, and such administration achieves, for example, full suppression of type 1 diabetes.

In another embodiment of the present invention, the MHC complex comprises the MHC Class II molecule.

In one embodiment of the present invention, the composition comprises Ig-INSβ, Ig-GAD1, IgGAD2 or an immunoglobulin or a portion thereof linked to a peptide derived from GAD65.

In one embodiment, the composition is endocytosed (or capable of being endocytosed) by cells having an Fe receptor and is processed and presented by the cells in association with MHC class II molecules thereby substantially reducing or preventing activation of diabetogenic T cells.

In another embodiment of the present invention, the T cells are antigen specific.

In one embodiment of the present invention, a composition is provided comprising an immunoglobulin or portion thereof linked to a protein fragment or peptide wherein the immunoglobulin or portion thereof is capable of binding to an Fc receptor, the peptide being selected from peptides derived from INS and GAD and more specifically INSβ, GAD 1 and GAD2. In a related embodiment, the composition has the property of being endocytosed by cells bearing the Fe receptor and processed and presented by the cells to present the peptide to endogenous MHC Class II molecules, thereby substantially reducing or preventing activation of diabetogenic T cells specific for the peptide.

In another embodiment, the composition is selected from the group consisting of agg Ig-INSβ and soluble Ig-INSβ.

In one embodiment, the peptide is a T cell receptor engaging determinant. In another embodiment, the peptide is inserted within the variable region of the immunoglobulin or portion thereof. In one embodiment, the peptide is inserted within the region selected from the group consisting of CDR1, CDR2 and CDR3.

In another embodiment, the immunoglobulin or portion thereof is human IgG or derived from human IgG or humanized IgG.

In another embodiment, the immunoglobulin or portion thereof is in an aggregated form. In another embodiment of the present invention, the immunoglobulin or portion thereof is in soluble form.

In another embodiment, the composition further comprises a pharmaceutically acceptable carrier.

In another embodiment, a use of a composition is provided wherein the composition comprises an immunoglobulin or portion thereof linked to one or more peptides wherein the immunoglobulin or portion thereof is capable of binding to an Fc receptor and being endocytosed by an antigen presenting cell and the one or more peptides or fragments thereof provides a T cell receptor antagonist for presentation on the surface of the antigen presenting cell upon endocytic processing for the preparation of a pharmaceutical composition for alleviating symptoms associates with type 1 diabetes for a patient in need.

In another embodiment, the immunoglobulin or portion thereof is comprised of at least part of a domain of a constant region of an immunoglobulin.

In one embodiment, the provided T cell receptor engaging determinant or epitope is presented on the surface of the antigen presenting cells associated with at least one MHC complex.

IL-10's function in diabetes is dependent on a number of factors (24-29). Systemic IL-10 has been shown to prevent diabetes in NOD mice while local production of IL-10 accelerated the development of disease in the NOD strain (24-26). As shown in the following Examples, agg Ig-INSβ was injected intraperitoneally and IL-10 was produced by APCs or “regulatory” T cells in a systemic manner; yet, diabetes was not delayed even though a peripheral tolerance mechanism by lack of costimulation was in place. In contrast, when agg Ig-INSβ was administered intraperitoneally at the pre-insulitis stage it was much more effective than the soluble form for suppression of diabetes (FIG. 9). The involvement of IL-10 in this pre-insulitis regimen is crucial as IL-10-deficient mice treated with agg Ig-INSβ displayed no delay of diabetes (FIG. 10). Thus, IL-10 appears to display a stimulatory function when its production is triggered after IAA-seroconversion but supports a modulatory function when produced at the pre-insulitis stage. One explanation for this observation is that encounter with IL-10 by diabetogenic T cells within the islets promote stimulation while exposure of the diabetogenic T lymphocytes prior to migration to the islets sustains modulation. Indeed, soluble Ig-INSβ given to mice after IAA-seroconversion supported delay and partial protection against diabetes indicating that diabetogenic T cells remain susceptible to tolerance while agg Ig-INSβ, which would also support peptide presentation with minimal or no costimulation but includes IL-10 production by APCs, had no protective effect.

At the age of 10 to 12 weeks, a time when the mice have seroconverted to become IAA-positive, insulitis is usually in place and diabetogenic T cells have already infiltrated the islets (4). However, these T cells, although vulnerable to treatment with soluble Ig-INSβ, seem to resist the aggregated form of the chimera. Since both aggregated and soluble forms of Igs do not up-regulate costimulatory molecules (20) but only the aggregated form induces IL-10 production by APCs, it is likely that diabetogenic T cells exposed to IL-10 within the islets resist tolerance. Indeed these cells were stimulated to produce IFNγ upon incubation with agg Ig-INSβ or even INSβ peptide and rIL-10 (FIG. 11).

It has been previously shown that local IL-10 produced within the islets up-regulates ICAM-1 on pancreatic vascular endothelium and facilitate acceleration of insulitis (24). At the pre-insulitis stage, the diabetogenic T cells may be exposed to IL-10 outside of the islets, most likely resulting in synergy with lack of costimulation leading to effective delay of diabetes. In fact, splenic T cells from 14 week old mice down-regulated IFNγ production when incubated with agg Ig-INSβ or INSβ and rIL-10 (FIG. 11). The notion that encounter of T cells with IL-10 prior to migration to the islets has a different outcome from encounters that happen within the islets is supported by studies demonstrating that delivery of IL-10 at a young age and before insulitis takes place delays diabetes (27, 48) while prevention of IL-10-IL-10R interactions before insulitis exacerbates the disease (28). Also, the observation bodes well with the modulatory function of transgenic and viral vector delivered IL-10, which would modulate T cells prior to migration to the islets (29, 49, 50). However, it remains unclear how injection of anti-IL-10 antibody at the pre-insulitis stage delays diabetes (27, 49) despite that agg Ig-INSβ treatment was unable to delay the disease in IL-10-deficient mice (see FIG. 10). Also, injection of anti-IL-10 antibody during treatment with agg Ig-INSβ at the pre-insulitis stage delayed the disease (not shown) and this function may be related to a cross-reactivity with other cytokines or molecules involved in regulation of the pathogenesis of diabetes (49). Since agg Ig-INSβ induced T cells producing TGFβ in addition to IL-10 (FIG. 6), it remains unclear how such a suppressive cytokine could not lead to a delay of diabetes.

Overall, the Ig delivery system of the present invention provides an approach that displays, under different circumstances, distinct modulatory functions and can be adapted to delay diabetes in a human or non-human patient before the development of insulitis, in pre-disposed individuals who have seroconverted and produce autoantibodies against one or more β-cell associated antigens, such as, for example, IAA-positive individuals. The Ig delivery system of the present invention can also lead to suppression of type 1 diabetes and reversal of the disease after a subject has become pre-diabetic.

While not intending to be bound by theory, research suggests that IL-10 can act as an immunosuppressive. It has now been discovered, however, that this function can be exploited against autoimmunity in the treatment of type 1 diabetes. Variable effects have been observed when IL-10 was utilized for suppression of type I diabetes. Herein, insulin β chain (“INSβ”) 9-23 peptide is genetically expressed on an immunoglobulin (Ig) chimera and the resulting Ig-INSβ facilitated control of endogenous IL-10 and analysis of its function against diabetes. Soluble (“sol”) Ig-INSβ supported efficient peptide presentation while aggregated (“agg”) Ig-INSβ cross-linked Fcγ receptors additionally triggering IL-10 production by the antigen presenting cells. Both forms were then tested for suppression of diabetes in NOD mice at the pre-insulitis stage and following seroconversion to insulin autoantibody (“IAA”) production. Soluble Ig-INSβ displayed dose dependent delay of diabetes when given at either stage. However, aggregated Ig-INSβ, which induced IL-10- and TGFβ-producing T cells, thus involving sustained endogenous IL-10, was protective against diabetes when given before development of insulitis but had no effect in predisposed mice positive for IAA. This discrepancy correlated with variable susceptibility to IL-10 among islet and peripheral pathogenic T cells. Thus, IL-10 synergizes with peripheral tolerance at the pre-insulitis stage while in IAA-positive mice, where islet infiltration is progressive, disease suppression is more effective in the absence of IL-10. Thus, it is contemplated herein that expression of diabetogenic peptide on Ig displays broad efficacy against the diverse T cell specificities responsible for diabetes in NOD mice.

To test this premise, the I-A^(g7)-restricted insulin beta chain (INSβ) 9-23 peptide (30, 31) was genetically engineered into the variable region of an IgG2b molecule and the soluble and aggregated forms of the resulting Ig-INSβ chimera were tested for presentation to diabetogenic T cells and suppression of diabetes before and after seroconversion into production of insulin-specific autoantibodies (IAA). The results indicate that soluble Ig-INSβ displays partial protection against diabetes both at the pre-insulitis stage and in IAA-positive animals while agg Ig-INSβ, which induced IL-10- and TGFβ-producing cells, is effective prior to but not after IAA-seroconversion. The asymmetrical function of endogenous IL-10 may be related to variable susceptibility of the diabetogenic T cells to the cytokine depending on whether exposure occurs before or after migration to the islets.

In one embodiment, present invention demonstrates that soluble Ig-INSβ, which does not induce IL-10 production upon binding to FcγRs, displays down-regulatory functions in vivo and delays the onset of diabetes in IAA-seropositive NOD mice (FIGS. 4, 5 and 7). Although complete suppression has not been achieved, the observed delay remains of great significance as the approach provides a means to treat predisposed subjects before the disease progresses to an irreversible stage. Also, continuous weekly administration of soluble Ig-INSβ can fully protect against the disease in IAA-positive mice. Because Ig-INSβ uses the same IgG2b isotype as Ig-PLP1 and Ig-MOG (22, 23) and like these chimeras may not induce the up-regulation of costimulatory molecules on APCs upon injection into animals free of adjuvant (20), the resulting INSβ presentation in vivo most likely lacks costimulatory leading to a peripheral tolerance-like mechanism effective against diabetogenic T cells. On the other hand, it is shown that agg Ig-INSβ, which cross-links FcγR, induces IL-10 production by APCs (FIG. 5). As a consequence, such IL-10 secretion by APCs led to down-regulation of IFNγ production by specific T cells that were engaged to the APCs through INSβ peptide derived from agg Ig-INSβ (FIG. 5). Moreover, agg Ig-INSβ stimulated the induction of IL-10- and TGFβ-producing T cells in vivo (FIG. 6). Yet, agg Ig-INSβ was unable to suppress diabetes or even sustain partial modulatory functions that usually arise as a consequence of peptide presentation with minimal or no costimulation in those IAA-positive mice (FIG. 7). Thus, mobilization of endogenous IL-10, whether by stimulation of APCs or induction of “regulatory” T cells in animals that have seroconverted to IAA production and initiated insulitis, seems to antagonize peripheral tolerance and support disease progression.

In one embodiment, compositions of the invention are formulated as an injectable formulation and comprise, for example, an aqueous solution or suspension of the active ingredient suitable for intravenous delivery. When preparing the composition for injection, particularly for intravenous delivery, a continuous phase can be present that comprises an aqueous solution of tonicity modifiers, buffered to a pH below about 7, or below about 6, for example about 2 to about 7, about 3 to about 6 or about 3 to about 5. The tonicity modifiers can comprise, for example, sodium chloride, glucose, mannitol, trehalose, glycerol, or other pharmaceutical agents that render osmotic pressure of the formulation isotonic with blood. Alternatively, when a larger quantity of the tonicity modifier is used in the formulation, it can be diluted prior to injection with a pharmaceutically acceptable diluent to render the mixture isotonic with blood.

In another embodiment of the present invention, compositions of the invention are in the form of solid dosage forms, for example tablets (including but not limited to swallowable tablets, chewable tablets, suspension tablets, etc.), capsules, caplets, troches, losenges, powders, granules, etc. Solid compositions are illustratively prepared by mixing the therapeutic agent with a pharmaceutical excipient to form a solid preformulation composition containing a homogeneous mixture of the therapeutic agent and excipient. When referring to these preformulation compounds as homogeneous, it is meant that the agents are substantially evenly distributed throughout the composition so that the composition may be readily subdivided into equally effective unit dosage forms, such as tablets, pills and capsules. This solid preformulation is then subdivided into unit dosage forms of the type described herein.

Compressed tablets are solid dosage forms prepared by compacting a formulation containing a therapeutic agent and excipient selected to aid the processing and improve the properties of the product. The term “compressed tablet” generally refers to a plain, uncoated tablet for oral ingestion, prepared by a single compression or by pre-compaction tapping followed by a final compression.

The solid dosage forms of the present invention may be coated or otherwise compounded to provide a dosage form affording the advantage of improved handling or storage characteristics. For example, a tablet or pill can comprise an inner dosage and an outer dosage component, the latter being in the form of an envelope over the former. In another embodiment, the compositions of the present invention are administered by intravenous (IV) infusion or intra-arterial administration over a desired period (for example, bolus injection, 5 min, 15 min, 30 min, 1 hr, 2 hr, 3 hr, 6 hr, 24 hr, 48 hr, 72 hr or 96 hour infusions). In one embodiment of the present invention the period of administration is no greater than about 3 hours.

Compositions of the present invention can further comprise one or more pharmaceutically acceptable excipients. Suitable excipients are any of those commonly used excipients in pharmaceutics and should be selected on the basis of compatibility with the pharmaceutical agent and the release profile properties of the desired dosage form. Any suitable excipient can be present in a composition of the invention in an amount of about 1% to about 80%, about 2% to about 70%, about 3% to about 60%, about 4% to about 50%, or about 5% to about 40%, by weight.

Illustrative classes of pharmaceutical excipients include binders, disintegrants, filling agents, surfactants, solubilizers, stabilizers, preservatives, lubricants, wetting agents, diluents, tableting agents, glidants, etc.

In one embodiment, a composition of the invention comprises a preservative. Illustrative preservatives includes benzalkonium chloride, propylparabem, butylparaben, chlorobutanol, benzyl alcohol, phenol, sodium benzoate, or EDTA.

Illustrative binders include acacia, alginic acid and salts thereof, cellulose derivatives, methylcellulose, hydroxyethyl cellulose, hydroxypropyl cellulose, magnesium aluminum silicate, polyethylene glycol, gums, polysaccharide acids, bentonites, hydroxypropyl methylcellulose, gelatin, polyvinylpyrrolidone, polyvinylpyrrolidone/vinyl acetate copolymer, crospovidone, povidone, polymethacrylates, hydroxypropylmethylcellulose, hydroxypropylcellulose, starch, pregelatinized starch, ethylcellulose, tragacanth, dextrin, microcrystalline cellulose, sucrose, or glucose, and the like.

Illustrative disintegrants (also referred to as disintegration agents) include starches, pregelatinized corn starch, pregelatinized starch, celluloses, cross-linked carboxymethylcellulose, sodium starch glycolate, crospovidone, cross-linked polyvinylpyrrolidone, croscarmellose sodium, a calcium, a sodium alginate complex, clays, alginates, gums, or sodium starch glycolate, and any disintegration agents used in solid preparations.

Illustrative filling agents include lactose, calcium carbonate, calcium phosphate, dibasic calcium phosphate, calcium sulfate, microcrystalline cellulose, cellulose powder, dextrose, dextrates, dextran, starches, pregelatinized starch, sucrose, xylitol, lactitol, mannitol, sorbitol, sodium chloride, polyethylene glycol, and the like.

Illustrative surfactants include sodium lauryl sulfate, sorbitan monooleate, polyoxyethylene sorbitan monooleate, polysorbates, polaxomers, bile salts, glyceryl monostearate, Pluronic™ line (BASF), and the like.

Illustrative solubilizers include citric acid, succinic acid, fumaric acid, malic acid, tartaric acid, maleic acid, glutaric acid sodium bicarbonate and sodium carbonate and the like.

Illustrative stabilizers such as antioxidation agents, buffers, or acids, and the like, can also be utilized.

Illustrative lubricants include magnesium stearate, calcium hydroxide, talc, sodium stearyl fumarate, hydrogenated vegetable oil, stearic acid, glyceryl behapate, magnesium, calcium and sodium stearates, stearic acid, talc, waxes, Stearowet, boric acid, sodium benzoate, sodium acetate, sodium chloride, DL-leucine, polyethylene glycols, sodium oleate, or sodium lauryl sulfate, and the like.

Illustrative wetting agents include oleic acid, glyceryl monostearate, sorbitan monooleate, sorbitan monolaurate, triethanolamine oleate, polyoxyethylene sorbitan monooleate, polyoxyethylene sorbitan monolaurate, sodium oleate, or sodium lauryl sulfate, and the like.

Illustrative diluents include lactose, starch, mannitol, sorbitol, dextrose, microcrystalline cellulose, dibasic calcium phosphate, sucrose-based diluents, confectioner's sugar, monobasic calcium sulfate monohydrate, calcium sulfate dihydrate, calcium lactate trihydrate, dextrates, inositol, hydrolyzed cereal solids, amylose, powdered cellulose, calcium carbonate, glycine, or bentonite, and the like.

Illustrative anti-adherents or glidants include talc, corn starch, DL-leucine, sodium lauryl sulfate, and magnesium, calcium, or sodium stearates, and the like.

Illustrative pharmaceutically compatible carriers include acacia, gelatin, colloidal silicon dioxide, calcium glycerophosphate, calcium lactate, maltodextrin, glycerine, magnesium silicate, sodium caseinate, soy lecithin, sodium chloride, tricalcium phosphate, dipotassium phosphate, sodium stearoyl lactylate, carrageenan, monoglyceride, diglyceride, or pregelatinized starch, and the like.

Additionally, drug formulations are discussed in, for example, Hoover, John E., Remington's Pharmaceutical Sciences, Mack Publishing Co., Easton, Pa. 1975. Another discussion of drug formulations can be found in Liberman, H. A. and Lachman, L., Eds., Pharmaceutical Dosage Forms, Marcel Decker, New York, N.Y., 1980.

In making compositions of the present invention, the individual components can be mixed with a pharmaceutically acceptable excipient, diluted by the excipient or enclosed within a capsule, sachet, paper or other container.

When an excipient serves as a diluent, it can be a solid, semi-solid or liquid material, which acts as a vehicle, carrier or medium for the active ingredient. Thus, the compositions can be in the form of a tablet, pill, powder, lozenge, sachet, cachet, elixir, troche, suspension, emulsion, solution, syrup, aerosol (as a solid or in a liquid medium), soft and hard gelatin capsule, sterile packaged powder, dispensable powder, granule, or liquid.

In one embodiment of the present invention, the manufacturing processes may employ one or a combination of methods: (1) dry mixing, (2) direct compression, (3) milling, (4) dry or non-aqueous granulation, (5) wet granulation, or (6) fusion. Lachman et al., The Theory and Practice of Industrial Pharmacy (1986). Such tablets may also comprise film coatings, which disintegrate upon oral ingestion or upon contact with diluent.

The present invention is also directed to a therapeutic method of treating a condition or disorder where treatment with an anti-diabetic type-I agent is indicated. The method comprises the administration of one or more of the pharmaceutical compositions of the present invention to a subject in need thereof. In one embodiment, the dosage regimen to prevent, give relief from, or ameliorate the condition or disorder corresponds to once-a-day or twice-a-day dosages, and can include, for example, about 0.0001 mg/kg, about 0.0005 mg/kg, about 0.001 mg/kg, about 0.01 mg/kg, about 0.05 mg/kg, about 0.1 mg/kg, about 0.5 mg/kg, about 1 mg/kg, about 2 mg/kg, about 5 mg/kg, about 10 mg/kg, about 15 mg/kg, about 20 mg/kg, about 30 mg/kg, about 40 mg/kg, about 50 mg/kg, about 60 mg/kg, about 70 mg/kg, about 80, mg/kg, about 90 mg/kg, about 100 mg/kg, about 110 mg/kg, about 120 mg/kg, about 130 mg/kg, about 140 mg/kg, about 150 mg/kg, about 160 mg/kg, about 170 mg/kg, about 180 mg/kg, about 190 mg/kg, about 200 mg/kg, about 220 mg/kg, about 240 mg/kg, about 250 mg/kg, about 500 mg/kg, about 750 mg/kg, or about 1,000 mg/kg (by body weight of the subject) dose of a therapeutic agent of the present invention, and can be modified in accordance with a variety of factors. These specific mg/kg amounts can vary, for example, from about 0.01% to about 20% or more, depending on the application and desired therapeutic result. Other factors include the type of subject, the age, weight, sex, diet, and medical condition of the subject and the severity of the disease. Thus, the dosage regimen actually employed can vary widely and therefore deviate from the dosage regimen set forth above.

In various embodiments, dosage units of the present invention contain, for example, about 1 ng to about 2000 mg; about 0.001 mg to about 750 mg, about 0.01 mg to about 500 mg, about 0.1 mg to about 300 mg or about 1 mg to about 100 mg of a therapeutic agent of the present invention. Illustratively, such unit dosage forms can contain about 0.001 mg, or about 0.01 mg, or about 0.1 mg, or about 1 mg, or about 2 mg, or about 5 mg, or about 10 mg, or about 15 mg, or about 20 mg, or about 30 mg, or about 40 mg, or about 50 mg, or about 60 mg, or about 70 mg, or about 80, mg, or about 90 mg, or about 100 mg, or about 110 mg, or about 120 mg, or about 130 mg, or about 140 mg, or about 150 mg, or about 160 mg, or about 170 mg, or about 180 mg, or about 190 mg, or about 200 mg, or about 300 mg, or about 400 mg, or about 500 mg, or about 750 mg, or about 1,000 mg of a therapeutic agent of the present invention.

Illustratively, dosage units each contain about 0.1 mg, about 1 mg, about 5 mg, about 10 mg, about 15 mg, about 20 mg, about 40 mg, about 80 mg, about 100 mg, about 250 mg, about 500 mg, or about 1000 mg of a therapeutic agent of the present invention. The dosage unit form can be selected to accommodate the desired frequency of administration used to achieve the specified daily dosage. In one embodiment, a composition of the invention will be administered to a subject in an amount sufficient to about 0.1 to about 15 mg, about 0.5 to about 10 mg, and or about 1 to about 5 mg of the active agent, for example soluble INSβ, sol Ig-GAD2, etc.

The amount of therapeutic agent necessary to elicit a therapeutic effect can be experimentally determined based on, for example, the absorption rate of the agent into the blood serum, the bioavailability of the agent, and the amount of protein binding of the agent. It is understood, however, that specific dose levels of the therapeutic agents of the present invention for any particular subject depends upon a variety of factors including the activity of the specific compound employed, the age, body weight, general health, sex, and diet of the subject (including, for example, whether the subject is in a fasting or fed state), the time of administration, the rate of excretion, the drug combination, and the severity of the particular disorder being treated and form of administration. Treatment dosages generally may be titrated to optimize safety and efficacy. Typically, dosage-effect relationships from in vitro and/or in vivo tests initially can provide useful guidance on the proper doses for subject administration. Studies in animal models generally may be used for guidance regarding effective dosages for treatment of diabetic disorders or diseases in accordance with the present invention. In terms of treatment protocols, it should be appreciated that the dosage to be administered will depend on several factors, including the particular agent that is administered, the route administered, the condition of the particular subject, etc. Generally speaking, one will desire to administer an amount of the compound that is effective to achieve a serum level commensurate with the concentrations found to be effective in vitro for a period of time effective to elicit a therapeutic effect. Thus, where a compound is found to demonstrate in vitro activity at, for example, 10 ng/ml, one will desire to administer an amount of the drug that is effective to provide at least about a 10 ng/ml concentration in vivo for a period of time that elicits a desired therapeutic effect, for example, lowering blood glucose level to acceptable levels, or improvement or elimination of symptoms, and other indicators as are selected as appropriate measures by those skilled in the art. Determination of these parameters is well within the skill of the art.

Initial treatment of a subject suffering from a condition or disorder where treatment with an anti-diabetic type 1 agent is indicated can begin with the dosages indicated above. Treatment is generally continued as necessary over a period of hours, days, weeks to several months or years until the condition or disorder has been controlled or eliminated. In one embodiment, a composition of the invention can be administered to a subject in a plurality of dosages. Illustratively, such administration can comprise a continuous (for example, by administration by an osmotic pump, patch, gel, cream, or infusion device), hourly, daily, weekly, bi-weekly, or monthly administration of the composition for any desired duration, for example for a period of about 1 week, about 2 weeks, about 1 month or more, about 3 months or more, about 6 months or more, about 9 months or more, about 1 year or more, about 3 years or more, about 5 years or more, or throughout the subject's life.

Subjects undergoing treatment with the compositions disclosed herein can be routinely monitored by any of the methods well known in the art to determine the effectiveness of therapy. Continuous analysis of such data permits modification of the treatment regimen during therapy so that optimal effective amounts of compounds of the present invention are administered at any point in time, and so that the duration of treatment can be determined as well. In this way, the treatment regimen/dosing schedule can be rationally modified over the course of therapy so that the lowest amount of an anti-diabetic type 1 agent exhibiting satisfactory effectiveness is administered, and so that administration is continued only so long as is necessary to successfully treat the condition or disorder.

The present methods, kits, and compositions can also be used in combination (“combination therapy”) with another pharmaceutical agent that is indicated for treating, preventing, suppressing or delaying the onset of type 1 diabetes, such as, for example, insulin, an alpha-glucosidase inhibitor, an insulin sensitizer, or a hyperglycemic agent, which are commonly administered to treat the symptoms and/or complications related to this disorder. These drugs have certain disadvantages associated with their use. Some of these drugs are not completely effective in the treatment of the aforementioned conditions and/or produce adverse side effects, such as hypoglycemia, microvascular disease, and macrovascular disease. However, when used in conjunction with the present invention, that is, in combination therapy, many if not all of these unwanted side effects may be reduced or eliminated. The reduced side effect profile of these drugs is generally attributed to, for example, the reduce dosage necessary to achieve a therapeutic effect with the administered combination.

The phrase “combination therapy” embraces the administration of a composition of the present invention in conjunction with another pharmaceutical agent that is indicated for treating or preventing type 1 diabetes in a subject, as part of a specific treatment regimen intended to provide a beneficial effect from the co-action of these therapeutic agents for the treatment of type 1 diabetes. The beneficial effect of the combination includes, but is not limited to, pharmacokinetic or pharmacodynamic co-action resulting from the combination of therapeutic agents. Administration of these therapeutic agents in combination typically is carried out over a defined time period (usually substantially simultaneously, minutes, hours, days, weeks, months or years depending upon the combination selected). “Combination therapy” generally is not intended to encompass the administration of two or more of these therapeutic agents as part of separate monotherapy regimens that incidentally and arbitrarily result in the combinations of the present invention. “Combination therapy” is intended to embrace administration of these therapeutic agents in a sequential manner, that is, where each therapeutic agent is administered at a different time, as well as administration of these therapeutic agents, or at least two of the therapeutic agents, in a substantially simultaneous manner. Substantially simultaneous administration can be accomplished, for example, by administering to the subject a single injection, tablet or capsule having a fixed ratio of each therapeutic agent or in multiple, single injections, capsules, or tablets for each of the therapeutic agents. Sequential or substantially simultaneous administration of each therapeutic agent can be implemented by any appropriate route. For example, the composition of the present invention can be administered orally, percutaneously, intravenously, intramuscularly, and/or directly absorbed through mucosal membranes while the other therapeutic agent of the combination can be administered by any appropriate route for that particular agent, including, but not limited to, an oral route, a percutaneous route, an intravenous route, an intramuscular route, or by direct absorption through mucous membrane tissues. The sequence in which the therapeutic agents are administered is not narrowly critical. “Combination therapy” also can embrace the administration of the therapeutic agents as described above in further combination with other biologically active ingredients, such as, but not limited to, (1) antiinflammatory agents, such as a steroidal or nonsteroidal antiinflammatory drug, and/or a 5-lipoxygenase inhibitor; or (2) an agent for treating cardiovascular disease or disorders, such as, for example, an antihypertensive agent, including, for example, an angiotensin converting enzyme inhibitor (ACE-inhibitor), an alpha-adrenergic agonist, a beta-adrenergic agonist, an alpha-adrenergic blocker, an angiotensin II receptor antagonist; a diuretic, including, for example, an aldosterone antagonist, a benzothiadiazine derivative, an organomercurial, a purine, a steroid (for example, canrenone, oleandrin, spironolactone), a sulfonamide derivative, or a uracil; an antianginal agent; an antiarrhythmic agent; an antiarteriosclerotic agent; an antihyperlipoproteinemic agent; an anicholelithogenic agent; an anticholesteremic agent; an antihypercholesterolemic agent; an antihyperlipidemic agent; an antihypertensive agent; an antihypotensive agent; an antilipidemic agent; a calcium channel blocker; a cardiac depressant agent; a dopamine receptor agonist; a dopamine receptor antagonist; a HMG CoA reductase inhibitor; an hypocholesteremic agent; a hypolipidemic agent; a hypotensive agent; a monoamine oxidase inhibitor; a muscle relaxant; a potassium channel activator; a pressor agent; a serotonin uptake antagonist; a thrombolytic agent; a vasodilator agent; a vasopressor agent; or a vasoprotectant agent (Based in part upon the list provided in The Merck Index, Merck & Co. Rahway, N.J. (2001), which is hereby incorporated by reference); and with non-drug therapies, such as, but not limited to, surgery.

The therapeutic compounds which make up the combination therapy may be a combined dosage form or in separate dosage forms intended for substantially simultaneous administration. The therapeutic compounds that make up the combination therapy may also be administered sequentially, with either therapeutic compound being administered by a regimen calling for two step administration. Thus, a regimen may call for sequential administration of the therapeutic compounds with spaced-apart administration of the separate, active agents. The time period between the multiple administration steps may range from, for example, a few minutes to several hours to days, depending upon the properties of each therapeutic compound such as potency, solubility, bioavailability, plasma half-life and kinetic profile of the therapeutic compound, as well as, depending upon the effect of food ingestion and the age and condition of the subject. Circadian variation of the target molecule concentration may also determine the optimal dose interval. The therapeutic compounds of the combined therapy whether administered simultaneously, substantially simultaneously, or sequentially, may involve a regimen calling for administration of one therapeutic compound by oral route and another therapeutic compound by an oral route, a percutaneous route, an intravenous route, an intramuscular route, or by direct absorption through mucous membrane tissues, for example. Whether the therapeutic compounds of the combined therapy are administered orally, by inhalation spray, rectally, topically, buccally (for example, sublingual), or parenterally (for example, subcutaneous, intramuscular, intravenous and intradermal injections, or infusion techniques), separately or together, each such therapeutic compound will be contained in a suitable pharmaceutical formulation of pharmaceutically-acceptable excipients, diluents or other formulations components.

The term “prevent” or “prevention,” in relation to a type 1 diabetic disorder or disease, means no type 1 diabetic disorder or disease development if none had occurred, or no further type 1 diabetic disorder or disease development if there had already been development of the disorder or disease.

The term “suspend” or “suspending” or “suspending the onset of” in relation to a type 1 diabetic disorder or disease refers to increasing time to clinical onset of diabetes for a given subject or group of subjects. Diabetes or the onset of diabetes can be determined by any method known in the art. (See, for example, The American Diabetes Association at http://www.diabetes.org/homepage.jsp). Illustratively, onset of diabetes in a human subject will be determined on the basis of high levels of urine or serum glucose as compared to a normal subject by using, for example, a urine glucose level test or a fasting plasma glucose test, respectively. In the fasting plasma glucose test, a subject will fast overnight (for example, at least about 8, 12, 16, or 24 hours) and a sample of the subject's blood will be drawn in the morning. Typically, normal fasting plasma glucose levels are less than about 110 milligrams per deciliter (mg/dl). Fasting plasma glucose levels of more than about 126 mg/dl on two or more tests on different days indicate development of a type I diabetic disorder or disease.

In another embodiment, onset of diabetes can be determined randomly by testing blood glucose levels taken shortly after eating or drinking. Blood glucose levels greater than about 200 mg/dl indicates diabetes, and can be confirmed with another test, such as, a fasting plasma glucose test or an oral glucose tolerance test. In an oral glucose tolerance test, a subject undergoes a fast of at least about 8 to 16 hours and is then administered about 75 grams of glucose (or 100 grams for a pregnant women). Blood samples are taken over a period of about 2 to 3 hours. In one embodiment, in a subject where blood glucose levels rise higher than normal (for example, blood glucose levels greater than 200 mg/dl between 0 to 2 hours, or greater than about 140 mg/dl at 2 hours) the subject is diagnosed with impaired glucose tolerance. In another embodiment, the present invention provides methods for preventing, delaying or reversing type 1 diabetes in a subject with a fasting blood sugar greater than about 126 mg/dl or a subject with a blood sugar of about 140 to about 200 mg/dl, post prandial. In another embodiment, the present invention provides methods for preventing, delaying or reversing type 1 diabetes in a subject that meets the following criteria: after ingestion of 75 g of glucose, venous plasma glucose concentration at 2 h is about 140 to about 200 mg/dl, and on at least one other occasion during the 2 hour test plasma glucose tolerance is equal to or greater than 200 mg/dl.

In another embodiment, a subject is confirmed to have diabetes when two or more diagnostic tests are done on different days that shows that blood glucose levels are higher than normal for the particular subject. The particular test used may vary to confirm the delay of onset of diabetes and will generally be interpreted on a subject-by-subject basis determined by those skilled in the art. For example, in an adult women, gestational diabetes may be diagnosed when one or more of the following results are positive: (i) a fasting (for example, at least 8 hours) blood glucose level greater than about 95 mg/dl; (ii) a one-hour glucose level greater than about 180 mg/dl; (iii) a two-hour glucose level greater than about 155 mg/dl; or (iv) a three-hour glucose level greater than about 140 mg/dl. Another test useful in the present invention commonly used by those skilled in the art to diagnose impaired glucose tolerance or diabetes is the glycated hemoglobin test, or A1C test.

In one embodiment, the present invention provides a method for reversing diabetes in a subject, for example a human subject, in need thereof, the method comprising the steps of: (a) diagnosing the subject as having diabetes; and (b) administering to the subject a composition of the invention as are described herein. Optionally, the method further comprises a step of monitoring blood glucose levels in the subject at one or more time points after administration. In one embodiment, the above treatment restores normoglycemia. In another embodiment, normoglycemia is restored without exogenous insulin or stem cell infusion. In another embodiment, normoglycemia is restored in conjunction with exogenous insulin and/or stem cell therapy.

In another embodiment, the present invention provides a method for regenerating endogenous beta cells in a subject, for example a human subject, in need thereof, the method comprising the steps of: (a) diagnosing the subject as being in need of beta cell regeneration or as having diabetes; and (b) administering to the subject a composition of the invention as is described herein. Optionally, the method further comprises a step of measuring beta cell regeneration or insulin production.

The term “pharmaceutically-effective amount” in relation to the amount of an agent to treat type 1 diabetes means, consistent with considerations known in the art, the amount of a type 1 diabetic agent effective to elicit a pharmacologic effect or therapeutic effect (including, but not limited to, reducing and/or controlling hyperglycemia), without undue adverse side effects.

The term “treat” or “treatment” as used herein refers to any treatment of a disorder or disease associated with type 1 diabetes, and includes, but is not limited to, preventing the disorder or disease from occurring in a subject which may be predisposed to the disorder or disease, but has not yet been diagnosed as having the disorder or disease; inhibiting the disorder or disease, for example, arresting the development of the disorder or disease; relieving the disorder or disease, for example, causing regression of the disorder or disease; relieving the condition caused by the disease or disorder, for example, stopping the symptoms of the disease or disorder, and/or delaying the onset of the disease or disorder. For example, treatment of a subject include reducing blood glucose levels in a hyperglycemic subject, and/or maintaining acceptable control of blood glucose levels in the subject. Such treatment, prevention, symptoms and/or conditions can be determined by one skilled in the art and are described in standard textbooks.

In another embodiment, a composition of the present invention is packaged in the form of a kit containing one or more of the compositions or therapeutic agents of the present invention. The kit can comprise hourly, daily, weekly, or monthly (or other periodic) dosages and can be arranged for proper sequential or simultaneous administration. The present invention further provides a kit or package containing a plurality of dosage units, adapted for successive daily administration, each dosage unit comprising at least one of the compositions or therapeutic agents of the present invention. This drug delivery system can be used to facilitate administration of any of the various embodiments of the compositions and therapeutic agents of the present invention. In one embodiment, the system contains a plurality of doses to be to be administered daily or as needed for symptomatic relief. The kit or package can also contain agents utilized in combination therapy to facilitate proper administration of the dosage forms. The kit or package can also contain a set of instructions for the subject.

EXAMPLES

The present invention is further illustrated by the following examples, which should not be construed as limiting in any way. The materials and methods as used in the following experimental examples are described below.

NOD (H-2^(g7)) mice were purchased from Jackson Laboratories (Bar Harbor, Me.) and IL-10-deficient (IL-10^(−/−)) NOD mice were previously described (32) and are also available from Jackson Laboratories. All mice were maintained in an animal facility for the duration of experiments and the experimental procedures performed on these animal were carried out according to the guidelines of the institutional animal care committee.

Assessment of diabetes

Mice are bled from the tail vein weekly and the blood samples are used to assess for both glucose content and anti-insulin antibodies. For measurement of glucose, a drop of blood is directly placed on a test strip and the glucose content is read using an Accu-Chek Advantage monitoring system (Roche Diagnostics, Indianapolis, Ind.). For detection of anti-insulin antibodies the blood is allowed to coagulate for 1 hour at room temperature and the serum is separated and used for ELISA. A mouse is considered diabetic when the blood glucose is above 300 mg/dl for two consecutive weeks.

Peptides

All peptides used in this study were purchased from Research Genetics, Inc. (Huntsville, Ala.) and purified by HPLC to >90% purity. INSβ peptide (Seq. I.D. No. 1 [SHLVEALYLVCGERG]) encompasses a diabetogenic epitope corresponding to amino acid residues 9-23 of the insulin β chain (30, 31). Hen egg lysozyme (“HEL”) peptide (Seq. I.D. No. 2 [AMKRHGLDNYRGYSL]) encompasses a non-diabetogenic epitope corresponding to amino acid residues 11-25 of HEL. Both INSβ and HEL peptides are presented to T cells in association with I-Ag^(g7) MHC class II molecules (30, 33). Other peptides that may be inserted within the variable region within the CDR region of an Ig and utilized for creating compositions for the treatment of type 1 diabetes as taught in the present invention are: GAD1 (Glutamic acid decarboxylase-65 also known as “GAD65”); corresponding to amino acid residues 524-543 of GAD 65 (Seq. I.D. No. 3 [SRLSKVAPVIKARMMEYGTT]) to create chimera Ig-GAD1; and 2) GAD2; corresponding to amino acid residues 206-220 of GAD 65 (Seq. I.D. No. 4 [TYEIAPVFVLLEYVT]); and other peptides derived from GAD65.

Other peptides derived from GAD or the human insulin protein (alpha and beta chains) are within the scope of the present invention. The peptides are often referred to herein as a “T cell receptor engaging determinant or epitope” in that they may work as an agonist or an antagonist or may interfere with the T cell receptor in another manner.

Ig Chimeras

Ig-INSβ is a chimera expressing INSβ peptide, which corresponds to amino acid residues 9-23 of insulin β chain. Construction of Ig-INSβ 3 used the genes coding for the heavy and light chains of the anti-arsonate antibody, 91A3, according to the procedures described for the construction of Ig-PLP1 (18, 34). In brief, the 91A₃V_(H) gene was subcloned into the EcoRI site of a pUC19 plasmid and used as template DNA in PCR mutagenesis reactions to generate 91A3V_(H) fragments carrying the INSβ (91A₃V_(H)-INSβ) sequence in place of the D segment within complementarity determining region 3 (CDR3). The 91A3V_(H)-INSβ fragment was then subcloned into an expression vector in front of the exons coding for the constant region of a BALB/c γ2b (18). This plasmid was then co-transfected into the non-Ig-producing SP2/0 myeloma B cell line with an expression vector carrying the parental 91A3 light chain. Transfectants producing Ig-INSβ were selected in the presence of geneticin and mycophenolic acid. Ig-HEL, which encompasses amino acid residues 11-25 of HEL, was constructed using the same 91A3 genes according to the procedure described for Ig-INSβ. Both chimeras are made of identical heavy and light chain but carry different peptides. Ig-W, the parental 91A3 Ig (encoded by wild-type genes) not encompassing any foreign peptide, has been described elsewhere (18). Large-scale cultures of transfectoma cells were carried out in DMEM media containing 10% iron-enriched calf serum (BioWhittaker, Walkersville, Md.). Purification of Ig-INSβ, Ig-HEL, and Ig-W was carried out on separate columns of rat anti-mouse-kappa chain mAb coupled to CNBr-activated 4B sepharose (Amersham Pharmacia Biotech, Piscataway, N.J.).

It is also within the scope of the invention that the immunoglobulin or portion thereof has more than one peptide linked to the immunoglobulin. Furthermore, the immunoglobulin, or a portion thereon, can be human or humanized, such as, for example, human IgG, such as IgG1, IgG2, IgG2a, IgG2b, IgG3 and/or IgG4. The Ig-P chimeras of the present invention may also comprise a pharmaceutically acceptable carrier.

Aggregation of the Ig Chimeras

The chimeras were aggregated by precipitation with 50%-saturated (NH₄)₂SO₄ as has been previously described (22). In brief, filtered 100% saturated (NH₄)₂SO₄ was added at an equal volume to the Ig chimera preparation. The mixture was incubated at 24° C. for 1 hour with gentle agitation every 20 minutes. Subsequently, the samples were spun down at 10,000 rpm, and the pellet was resuspended at 1 mg/ml in PBS. Electrophoresis on a 10% acrylamide gel confirmed that the Ig chimera preparation was in aggregate form. Since both Ig-INSβ and Ig-HEL derive from the same Ig backbone and thereby comprise identical IgG2b isotype, their Fc associated functions will be similar.

Radioimmunoassay (RIA)

Capture RIA was used to assess secretion of complete Ig-INSβ and Ig-HEL constructs from SP2/0 transfectants. Microtiter 96-well plates were coated with polyclonal rabbit anti-mouse-γ2b chain specific antibody (Zymed Laboratories, South San Francisco, Calif.) (2 μg/ml in PBS) overnight at 4° C. and then blocked with 2% BSA in PBS for 1 hour at room temperature. The plates were then washed three times with PBS and 100 μl/well of supernatant from SP2/0 cells growing in the presence of selective drugs was incubated for 2 hours at room temperature. After three washes with PBS, captured Ig-chimeras were revealed by incubation with 1×10⁵ cpm/well ¹²⁵I-labeled rat anti-mouse kappa mAb (ATCC, Rockville, Md.) for 2 hours at 37° C. The plates were then washed five times with PBS and counted using a Wallac LKB gamma counter.

Generation of T Cell Lines and Hybridomas

T cell lines: A T cell line specific for INSβ peptide was generated by immunizing NOD mice with 100 μg of INSβ peptide in 200 μl PBS/CFA (vol/vol) subcutaneously (“s.c.”) in the footpads and at the base of each limb. After 10 days, the draining lymph nodes were removed, and T cells were stimulated in vitro for 2 rounds in the presence of irradiated (3000 rads), syngenic splenocytes, 5% T-Stim supplement (Collaborative Biomedical Products, Bedford, Mass.), and INSβ peptide (25 μg/ml). The culture media used to carry out these stimulations and other T cell activation assays in this study was DMEM supplemented with 10% FCS (Hyclone, Logan, Utah), 0.05 mM 2-mercaptoethanol, 2 mM glutamine, 1 mM sodium pyruvate, and 50 μg/ml gentamycin sulfate. NOD mice were also used for immunization with HEL peptide and generation of T cell line specific for HEL according to procedures similar to the INSβ specific line.

T cell hybridomas: A HEL-specific T cell line was fused with the αβ TCR negative thymoma BW1100 (ATCC) using polyethylene glycol 4000 (Sigma, St. Louis, Mo.). Hybrids were then selected by supplementing the culture media with hypoxanthine-azaserine (Sigma). Resulting hybridomas were then screened for reactivity to HEL peptide by testing for production of IL-2 in the supernatant following stimulation with irradiated (3000 rads) splenocytes in the presence of 15 μg/ml HEL peptide. Positive hybridomas were then cloned by limiting dilution and used to assess presentation of HEL peptide and Ig-HEL chimera.

Detection of Insulin Autoantibodies.

Detection of insulin autoantibodies (“IAA”) in the serum of NOD mice was carried out by ELISA as follows: microtiter plates number 3369 (Corning Inc, Corning, N.Y.) were coated with 50 μl sodium bicarbonate solution (pH 9.6) containing 10 μg/ml porcine insulin (Sigma, Saint Louis, Mo.) for 16 hours at 4° C. The plates were then washed 3 times with PBS-0.05% Tween-20 and free plastic sites were saturated by incubation with 2.5% Casein (in 0.3M NaCl pH 7) for 2 hours at RT. Subsequently, serum samples ( 1/200 dilutions) were added and the plates were incubated for 16 hours at 4° C. Biotin-conjugated rat anti-mouse kappa mAb (100 μl at 1 μg/ml) was added and the plates were incubated for 1 hour at RT. Bound anti-mouse Kappa mAb was revealed by incubation with a casein solution containing 2.5 mg/ml avidin peroxidase for 30 min at RT followed by addition of ABTS substrate. The samples were read at 405 nm on a Spectramax 190 (Molecular Devices, Sunnyvale, Calif.)

Regimens for Suppression of Diabetes

Treatment of IAA-positive NOD mice with Ig-INSβ: Preliminary studies were carried out and indicated that seroconversion to IAA-positive occurs most frequently between the ages of 8 and 12 weeks. Mice are given weekly intraperitoneal injections of soluble or agg Ig-INSβ or Ig-HEL beginning the week of seroconversion. The mice were given either 2 or 3 injections 7 days apart of Ig chimera in 300 μl saline solution. Beginning at week 12 of age, the mice were tested weekly for blood glucose up to week 30 unless previously diagnosed diabetic.

Treatment of NOD mice with Ig-INSβ at the pre-insulitis stage: The mice were given a weekly i.p. injection of 300 μg Ig-INSβ or Ig-HEL in 300 μl saline beginning at week 4 for a total of 3 injections. Beginning at week 12 of age, the mice were tested weekly for blood glucose up to week 30 unless previously diagnosed diabetic.

Detection of Cytokines in Cell Cultures

Detection of IL-10 and IFNγ was performed according to BD Pharmingen's standard protocol. The capture Abs were as follows: rat anti-mouse IL-10, JES5-2A5 and rat anti-mouse IFNγ, R4-6A2. The biotinylated anti-cytokine Abs were as follows: rat anti-mouse IL-10, JES5-16E3 and rat anti-mouse IFNγ, XMG1.2. Both antibodies were purchased from BD Pharmingen (San Diego, Calif.). ELISA for the detection of active TGFβ was preformed using the human TGFβ₁ DuoSet kit (R&D systems, Minneapolis, Minn.) according to the manufacturer's instructions. Bound TGFβ was revealed using the TMB microwell peroxidase substrate system (Kirkegaard & Perry Laboratories, Gaithersburg, Mass.). All assays were read on a SpectraMAX 190 counter. Graded amounts of recombinant mouse IFNγ, IL-10, and TGFβ were included in all experiments for construction of standard curves. The cytokine concentration in culture supernatants was interpolated from the linear portion of the standard curve.

Measurement of T Cell Responses

Responses of T cell lines: Purified bulk, dendritic cells (“DCs”) were plated at 5×10⁴ cells/well/50 μl and incubated with graded amounts of soluble or agg Ig-chimeras (100 μl/well) for 1 hour. Subsequently, peptide-specific T cells (5×10⁴ cells/well/50 μl) were added, and the culture was continued for 24 h. Detection and quantification of cytokines were assessed by ELISA from 100 μl of culture supernatant as described above.

Responses of NOD splenic T cells upon treatment with Ig-INSβ: Splenic cells (1×10⁶ per well) which include both T lymphocytes and APCs were incubated with 30 μg INSβ peptide and T cell responses were analyzed. Cytokines were measured by ELISA after 48 hours of incubation as described above and proliferation was assessed by [³H] thymidine incorporation after 3 days. In this proliferation assay the cells were incubated in 96-well flat bottom plates with or without the stimulator for 3 days and 1 μCi [³H] thymidine was added per well, during the last 14.5 h of stimulation. The cells were then harvested on a Trilux 1450 Microbeta Wallac Harvester and incorporated [³H] thymidine was counted using the Microbeta 270.004 software (EG&G Wallac INC, Gaithersburg, Md.). A control media with no stimulator was included and used as background.

Isolation of Splenic Dendritic Cells

Splenic DCs were purified according to the standard collagenase/differential adherence method (35). Briefly, the spleen was disrupted in a collagenase solution, and isolated DCs floated on a dense BSA gradient. Subsequently, the cells were allowed to adhere to petri dishes for 90 minutes at 37° C., washed, and incubated overnight. The DCs are then harvested and further purified on anti-CD11c coupled microbeads according to Miltenyi's instructions.

Stimulation of cytokine production by dendritic cells

Purified splenic CD11c⁺ DCs from NOD mice were plated with graded amounts of soluble or agg Ig chimeras, and the culture was then incubated for 24 h with or without specific T cells. Detection and quantification of cytokines was then assessed by ELISA from 100 μl of culture supernatant as described above.

Isolation of Islet-Infiltrating Lymphocytes

Islet-infiltrating cells were derived from 14 week old female NOD mice by collagenase digestion as previously described (36). Briefly, pancreata were collected in a PBS solution containing 5% FCS and 1% glucose, finely minced, and digested in a collagenase type IV (Invitrogen Corp., Carlsbad, Calif.) solution supplemented with 15% FCS for 8 min at 37° C. Islets were then pressed through a 100 μm metal sieve and successively filtered through 70 μm and 40 μm nylon screens to recover infiltrating cells. Viability of the cells was determined by trypan blue exclusion.

Example 1 Expression of INSβ and HEL Peptides on Ig Molecules Drives Efficient Presentation to T Cells

Recent studies have revealed that mice with an ongoing EAE ameliorate their disease when treated with chimeric Igs expressing myelin epitopes (20, 22, 23). This investigation seeks to determine whether similar delivery of a diabetogenic peptide on Igs could inhibit type-1 diabetes in the NOD mouse. The I-A⁶⁷-restricted INSβ peptide defined to be associated with the development of diabetes in the NOD mouse (37, 38) was selected for expression on Igs to generate an Ig-INSβ chimera suitable for evaluation against diabetes. HEL peptide, which is presented by I-Ag^(g7) MHC class II molecules without causing diabetes (30), was used to generate an Ig-HEL chimera to serve as a control. Accordingly, INSβ and HEL nucleotide sequences were separately inserted into the CDR3 of the 91A3 heavy chain by PCR mutagenesis (18) and the resulting chimeric heavy chain genes were analyzed by DNA sequencing (see “Materials and Methods”).

The results presented in FIG. 1 show the nucleotide sequences of these inserts as well as the flanking regions surrounding them. The top panel shows a comparison of the nucleotide sequence of the parental 91A₃V_(H) gene to the sequences of the chimeric 91A₃V_(H)-INSβ and 91A₃V_(H)-HEL. Both chimeric 91A3V_(H)-INSβ and 91A3V_(H)-HEL fragments were subcloned into an expression vector in front of the exons coding for the constant region of a BALB/c γ2b. The plasmids were then separately co-transfected into the non-Ig-producing SP2/0 myeloma B cell line with an expression vector carrying the parental 91A3 light chain. Transfectants producing Ig-INSβ were selected in the presence of geneticin and mycophenolic acid as described in the “Materials and Methods” (“Ig Chimeras”) (18). In the lower panel detection of secreted chimeric Ig in the supernatant from transfectoma cells was carried out by incubation of supernatant of Ig-INSβ, Ig-HEL or Ig-W transfectants on microtiter plates coated with rabbit anti-mouse γ2b -chain specific antibody and revelation of captured Ig-chimeras with [¹²⁵I]-labeled rat anti-mouse kappa light chain mAb. Each bar represents the mean ±SD of triplicates.

The data indicate that the INSβ nucleotide sequence was fully inserted in place of the D segment. The flanking regions surrounding INSβ are identical to those regions flanking the D segment within the parental heavy chain indicating that the INSβ nucleotide sequence was inserted in the correct reading frame. Similar results were obtained with HEL peptide indicating that a full nucleotide sequence of HEL peptide was incorporated in the correct reading frame. Subsequently, these chimeric heavy chain genes were subcloned into a pSV2 expression vector and separately co-transfected with the parental 91A3 kappa light chain gene into the non-Ig-secreting myeloma B cell line SP2/0 (18) and as taught in the “Materials and Methods” (“Ig Chimeras”).

Using selective drugs, the wells with cell growth were identified visually, and their supernatants were tested for the presence of Igs. As depicted in the lower panel of FIG. 1, supernatant from a representative Ig-INSβ transfectant incubated on plates coated with anti-γ2b antibody bound a rat anti-mouse kappa light chain mAb, as did Ig-W, the parental 91A3 antibody with an intact CDR3 domain indicating that the 91A3-INSβ chimeric heavy chain paired with the parental light chain and formed a complete Ig-INSβ molecule. Similarly, a representative supernatant from a 91A3-HEL transfectant showed significant binding of the anti-light chain antibody indicating that insertion of the HEL peptide within the heavy chain variable region did not alter pairing with the parental light chain and a complete Ig-HEL molecule was produced.

Example 2 Ig-INSβ is Processed Properly and Generates an INSβ Peptide that Could be Presented to T Cells

The next question to address was whether Ig-INSβ is processed properly and generates an INSβ peptide that could be presented to T cells. To test this premise, the chimera was purified from the supernatant of large-scale cultures by affinity chromatography and assayed for presentation using an INSβ-specific T cell line that has been generated in NOD mice by immunization with INSβ peptide (see “Materials and Methods”). Similarly, to ensure that HEL peptide could be processed from Ig-HEL and presented to T cells, an HEL-specific hybridoma was generated by fusing the HEL-specific short-term T cell line with the αβ-T cell receptor (αβ-TCR)-negative thymoma BW1100 (see “Material and Methods”).

Presentation of Ig-INSβ chimera to specific T cells was then determined. Irradiated (3000 rads) NOD splenocytes (5×10⁵ cells/50 μl/well) were incubated with 100 μl antigen and one hour later T cells (5×10⁴ cells/well/50 μl) specific for either INSβ (FIG. 2(a)-2(b)) or HEL (FIG. 2(c)-2(d 0) peptide were added. For presentation of INSβ peptide and Ig-INSβ (FIGS. 2(a) and 2(b) respectively), the activation was assessed by [³H] thymidine incorporation since, the T cells were from a line. Accordingly, 1 μCi [³H]thymidine per well was added during the last 14 hours of a 3-day incubation period and the cells were harvested, and the radioactivity counted. For presentation of HEL peptide (FIG. 2(c)) and Ig-HEL (FIG. 2(d)), T cell activation was assessed by measuring IL-2 production as the HEL-specific cells were from a hybridoma. Accordingly, after 24 hours incubation IL-2 was measured in 100 μl supernatant by ELISA. In this assay the peptides were used at 10 μM concentration and the Ig-chimeras at 1 μM. Each point or bar represents the mean of triplicates.

As indicated in FIG. 2, the INSβ-specific T cell line proliferated significantly upon incubation with irradiated NOD splenic APCs and INSβ peptide (FIG. 2(a)), or Ig-INSβ (FIG. 2(b)) indicating that Ig-INSβ is taken up by the APCs and an INSβ peptide is generated and presented to T cells. HEL peptide and Ig-HEL, although able to stimulate the HEL-specific hybridoma as measured by IL-2 production (FIGS. 2(c) and 2(d)), were unable to induce proliferation of the INSβ-specific line indicating that presentation of INSβ and Ig-INSβ is specific. The above described results demonstrate that INSβ and HEL peptide expressed on Igs are functional and suitable for evaluation of suppression of diabetes.

Example 3 Insulin-Specific Autoantibodies Can Serve as a Marker for Early Development of Diabetes

Gender study of the incidence of diabetes in our NOD colony indicated that 38% of male NOD mice develop spontaneous diabetes by the age of 26 weeks. However, female NOD mice have shown a greater susceptibility for the disease and 80% developed spontaneous diabetes at week 26 of age. This is in good agreement with previous reports and suggests that the use of female mice would be more suitable for our investigation.

Recently, it has been shown that IAA can be used as a marker for prediction of type I diabetes in children and young NOD mice (39, 40). This is advantageous as it targets intervention prior to significant destruction of β cells without compromising the accuracy of the study. Therefore, it was decided to develop a chart to include only IAA-positive mice to assess the ability of Ig-INSβ for suppression of diabetes. Accordingly, a group of 70 NOD female mice was subject to weekly testing for IAA beginning at week 6 through week 12 of age and the IAA-positive mice were monitored for blood glucose thereafter and up to 30 weeks.

In FIG. 3(a), 70 adult female NOD mice were bled weekly starting at the age of 6 weeks and their serum samples were tested for IAA at a 1/200 dilution by ELISA as described in the “Materials and Methods” section. A sample is considered IAA-positive when the OD₄₀₅ is >0.2. The cutoff of 0.2 was chosen because serum samples from 10 SJL mice, non-prone to diabetes development and presumably do not produce insulin specific autoantibodies, never exceeded 0.2 OD₄₀₅. Among the 70 mice tested, 58 (83%) have shown an IAA-positive result. In FIG. 3(b), the 58 mice that tested IAA-positive by week 12 were subjected to weekly measurement of blood glucose beginning at week 12 continuing through week 30. Among the 58 IAA-positive mice, 49 (84%) become diabetic by age 30 weeks. FIG. 3(c) shows the percent incidence of early (15-20 weeks of age) and delayed (21 to 30 weeks of age) diabetes for mice developing IAA at the indicated weeks. n indicates the number of mice per group.

As indicated in FIG. 3(a), the appearance of IAA begins at week 7 and by 12 weeks of age 58 among the 70 mice tested (83%) had become IAA-positive. Furthermore, among the 58 IAA-positive mice, 84% had become diabetic by 30 weeks of age (FIG. 3(b)) indicating that IAA can serve as a marker for the development of type I diabetes in female NOD mice. Interestingly, a significant percentage (60%) of the mice that became IAA-positive at week 8, 9, or 10 manifested diabetes at the age of 15 to 20 weeks and such early incidence rose to 80% for the mice who developed IAA at week 11 of age (FIG. 3(c)). Therefore, these results demonstrate suggest that development of IAA between the age of 8 to 11 weeks can serve as a marker for the development of diabetes at the early age of 15 to 20 weeks.

Example 4 Soluble Ig-INSβ Delays Diabetes when Administered into Mice upon IAA Seroconversion

Although infiltration of the pancreatic islets with inflammatory cells occurs long before hyperglycemia, pancreatic biopsy for histologic analysis represents an impractical approach for prediction of the onset of diabetes. Detection of IAA in blood samples is practical and has proven reliable for the prediction of early diabetes onset in the NOD mouse (39, 40). Thus, the IAA marker was used for evaluation of Ig-INSβ for suppression of diabetes before onset of hyperglycemia. Accordingly, NOD mice were tested for the presence of IAA and those who seroconverted at the age of 8 to 11 weeks were given soluble Ig-INSβ in saline on the week of seroconversion and thereafter as indicated, and monitored for blood glucose up to week 26 of age. Specifically, groups of female NOD mice (10 per group) positive for IAA between the age of 8 and 11 weeks were given an intraperitoneal (“i.p.”) injection of 100 μg (a), 200 μg (b), or 300 μg (c) of either soluble Ig-INSβ (black bars) or soluble Ig-HEL (hatched bars) on the week of seroconversion. All groups were given an additional injection of the same amount 7 days later and the mice in FIG. 4(c) received a third injection on day 14 after seroconversion. A seventh group did not receive any injection (Nil: open bars) and was incorporated in the three panels to serve as a control. The percentage incidence of diabetes is shown in each of the groups at week 19 and 26 of age in FIGS. 4(a)-4(c).

As can be seen in FIG. 4(a), two doses of 100 μg soluble Ig-INSβ had no significant delay on early onset diabetes and most of the animals became diabetic by week 26 of age. When two doses of 200 μg soluble Ig-INSβ were applied (FIG. 4(b)), the onset of diabetes was delayed and only 30% of the mice become diabetic by week 19 relative to 50% in the untreated group. Complete prevention was not achieved and by week 26 most of the soluble Ig-INSβ-treated animals developed diabetes. The delay of diabetes is antigen-specific as Ig-HEL had no significant delay or protection against diabetes. Increasing the dose to 300 μg per injection and giving a total of 3 injections delayed the early-onset diabetes significantly as only 20% of the mice developed diabetes by week 19 relative to 50% in the untreated group (FIG. 4(c)). Moreover, 50% of the soluble Ig-INSβ treated mice remained free of disease by week 26 of age while only 20% in the untreated group had no diabetes. The control Ig-HEL had no significant delay or protection against early or delayed diabetes.

Example 5 Administration of agg Ig-INSβ into NOD Mice Induces Antigen-Specific Non-Proliferative T Cells Producing Both IL-10 and TGFβ

Aggregation of Igs confers Fc associated functions such as cross-linking of FcγRs and activation of complement (41, 42). It has been previously shown that aggregation of Ig-myelin chimeras using the same IgG2b backbone as Ig-INSβ and Ig-HEL cross-links FcγRs on APCs and induces the production of IL-10 by both dendritic cells and macrophages (22, 23). In addition, while soluble Ig-myelin chimeras suppressed relapses with little effect on the initial severe phase of EAE, agg chimeras induced full and expeditious recovery from the initial paralytic phase and the relapses (20, 22). Neutralization of endogenous IL-10 by administration of anti-IL-10 antibody during treatment with the agg Ig-myelin chimeras restored disease severity (22). These results indicated that cross-linking of FcγRs and IL-10 production by APCs potentiate the modulatory function of Ig-myelin chimeras and promote effective suppression of EAE (20, 22). Such effectiveness may be due to synergy between endogenous IL-10 and myelin-peptide presentation with minimal costimulation (20). However, since IL-10 can serve as a growth factor for the development of regulatory T cells (43, 44), there may be induction of such cells that could support continuous production of IL-10 and provide additional modulatory functions against pathogenic T cells. To test whether similar effects could develop in the NOD system, Ig-INSβ was aggregated (see “Aggregation of Ig Chimeras” in “Materials and Methods”) and tested for induction of IL-10 by APCs, down-regulation of INSβ-specific T cell line in vitro and induction of IL-10 producing T cells in vivo.

In FIG. 5 a, purified NOD splenic DCs (5×10⁴ cells/well) were incubated with graded amounts of agg Ig-INSβ (closed circles) or soluble Ig-INSβ (open circles) and production of IL-10 was measured by ELISA 24 hours later. For down-regulation of INSβ-specific T cells (FIGS. 5 b-5 d), purified NOD splenic DCs (5×10⁴ cells/well) were incubated with graded amounts of agg Ig-INSβ (FIG. 5 b) or soluble Ig-INSβ (FIG. 5 c) for 1 h. Subsequently, the INSβ-specific T cell line TCL-INSβ-C1 (0.2×10⁵ cells/well) was added and incubation was continued for an additional 24 h. IL-10 (closed diamonds) and IFNγ (open diamonds) production in the same culture wells were then measured by ELISA from 100 μl of culture supernatant. Each point represents the mean of triplicate wells.

In FIG. 5 d, the assay was carried out in the absence (closed bars) or presence (open bars) of 40 μg/ml anti-IL-10 antibody or isotype control, rat IgG (hatched bars) with three different concentrations of agg Ig-INSβ. Each bar represents the mean±SD of triplicate wells.

The data shows that agg Ig-INSβ, which encompasses identical IgG2b isotype as the Ig-myelin chimeras, induced IL-10 production by DCs (FIG. 5 a). Soluble Ig-INSβ, however, was unable to trigger IL-10 production by the same DCs indicating that cross-linking of FcγRs is required for cytokine production. Moreover, IL-10, produced by the DCs upon presentation of agg Ig-INSβ, displayed down-regulatory functions on the activation of specific T cells engaged to the DCs through INSβ peptide. Indeed, when INSβ-specific T cells were incubated with DCs and agg Ig-INSβ, the secretion of IFNγ by the T cells decreased as production of IL-10 by the DCs increased (FIG. 5 b). Such down-regulation of IFNγ did not occur with soluble Ig-INSβ which did not induce IL-10 secretion by the DCs (FIG. 5 c). Neutralization of IL-10 during stimulation with agg Ig-INSβ restores IFNγ production by the T cells (FIG. 5 d).

Overall, these results indicate that agg Ig-INSβ drives both IL-10 production and peptide presentation by APCs which support down-regulation of INSβ-specific T cells.

Example 6 Agg Ig-INSβ Reduces Th1 Responses but Supports Production of IL-10 and TGFβ upon Administration into NOD Mice

Since IL-10 has been defined to function as a growth factor for the development of regulatory T cells (45, 46) that produce IL-10 (43, 47), agg Ig-INSβ (which triggers production of IL-10 by APCs) was tested for stimulation of non-proliferative cytokine producing T cells in vivo. Accordingly, splenic cells from mice given agg Ig-INSβ on week 4, 5 and 6 were harvested on week 12 and tested for proliferation and cytokine production upon in vitro stimulation with INSβ peptide. The rationale for testing the cells on week 12, rather than 10 days after completion of the treatment, is related to the fact that Ig-INSβ was injected without adjuvants and accumulation of suppressor cells may take a longer period of time. In addition, tolerization of pathogenic T cells needs to be advanced to minimize residual responses.

A Group of 5 untreated female NOD mice (gray bars, see FIG. 6) as well a group of 5 mice recipient of 300 μg agg Ig-INSβ at week 4, 5 and 6 of age (black bars, see FIG. 6) were sacrificed at 12 weeks and their splenic proliferative and cytokine responses were measured. In FIG. 6(a), pooled splenocytes (1×10⁶ cells/well) from 5 mice were stimulated with 30 μg/ml INSβ peptide for 72 h and proliferation was assessed as described in the “Materials and Methods” section. In FIGS. 6(b)-6(d), pooled splenocytes were stimulated with INSβ peptide for 48 h and cytokine production was assayed by ELISA using 100 μl of supernatant. Each bar represents the mean of triplicate wells.

The results illustrated in FIGS. 6(a)-6(d) indicate that proliferation is reduced in mice given Ig-INSβ relative to untreated animals and IFNγ has begun to decrease most likely due to down-regulation of diabetogenic T cells. Furthermore, an increase in IL-10 production accompanied by a selective secretion of TGFβ has been observed in the mice given agg Ig-INSβ relative to untreated mice. Overall, these results indicate that agg Ig-INSβ induces antigen-specific non-proliferative T cells producing both IL-10 and TGFβ.

Example 7 Agg Ig-INSβ Does Not Delay Diabetes when Administered into NOD Mice upon IAA Seroconversion

As agg Ig-INSβ induced IL-10 by APCs and stimulated T lymphocytes producing suppressive cytokines, it was expected the chimeras to be effective against diabetes in IAA-positive mice. Surprisingly, the results illustrated in FIG. 7 point to a different outcome.

Groups of female NOD mice (10 per group) positive for IAA between the age of 8 and 11 weeks were given an intraperitoneal injection of 100 μg [FIG. 7(a)], 200 μg [FIG. 7(b)], or 300 μg [FIG. 7(c)] of either agg Ig-INSβ (black bars) or agg Ig-HEL (hatched bars) on the week of seroconversion. All groups were given an additional injection of the same amount 7 days later and the mice in FIG. 7(c) received a third injection on day 14 after seroconversion. A seventh group did not receive any injection (Nil: open bars) and was incorporated in the three panels to serve as a control. FIGS. 7(a)-7(c) show the percentage incidence of diabetes in each of the groups at week 19 and 26 of age.

Testament with 2 doses of 100 μg agg Ig-INSβ did not delay the onset of early diabetes and consequently, no prolonged protection against the disease was observed. Increasing the dose to 200 μg per injection also did not induce significant delay of the onset of early diabetes and most of the mice developed hyperglycemia by week 26 of age. Injection of 300 μg agg Ig-INSβ once a week for 3 consecutive weeks did not significantly delay the onset of early diabetes and thus no long term protection against the disease had occurred.

Example 8 The Soluble Form of Ig-INSβ is More Effective Than the Aggregated Form in the Suppression of Diabetes in IAA-Positive Mice

As shown in FIG. 8, the bars represent the percentage of NOD mice that remained free of early (19 weeks) diabetes upon treatment with either agg Ig-INSβ or soluble Ig-INSβ. These percentages were generated according to the following formula: number of disease free animals in treated groups minus the number of disease free mice in the untreated group over the number of diabetic animals in the untreated group. These results were generated from the comparison of the mice recipient of 3 injections of 300 μg soluble Ig-INSβ (FIG. 4 c) or agg Ig-INSβ (FIG. 7 c).

These results are similar to those obtained with the control Ig-HEL. Overall, aggregated Ig-INSβ had little effect in delaying the onset of early or delayed diabetes. In fact, comparison of the soluble and aggregated forms of Ig-INSβ for suppression of diabetes after IAA seroconversion clearly shows that soluble Ig-INSβ significantly delays the onset of early diabetes and 60% of the mice were free of disease on week 19 (FIG. 8). In contrast, the aggregated form of Ig-INSβ, which brings IL-10 into the mechanism, had no statistically significant effect even in suppression of early diabetes.

Example 9 Agg Ig-INSβ is More Effective Than Soluble Ig-INSβ in Delaying the Onset of Diabetes When Administered at the Pre-Insulitis Stage

IL-10 has been shown to display contrasting effects on diabetes depending on the mode of delivery to the target cells (24-26). Similarly, IL-10-IL-10R interactions showed differential regulation of diabetes in young versus older animals (28). Since agg Ig-INSβ induces IL-10 production by APCs but did not suppress diabetes in IAA-positive animals while soluble Ig-INSβ, which does not induce IL-10 production, delayed diabetes, it was decided to investigate whether such differential effect on diabetes manifest when the chimeras are administered at the pre-insulitis stage.

Accordingly, NOD mice were given an injection of 300 μg of either agg or soluble Ig-INSβ at the age of 4 weeks and two additional injections (300 μg) at weeks 5 and 6, respectively, and the animals were monitored for blood glucose weekly up to week 26 of age. Groups of female NOD mice (10 per group) were given an i.p. injection of a saline solution containing 300 μg of soluble Ig-INSβ or agg Ig-INSβ (black bars), or Ig-HEL (hatched bars) at 4, 5 and 6 weeks of age (FIGS. 9(a)-9(b)). A fifth group that did not receive any injection (Nil: open bars) was included for control purposes. The mice were then monitored for blood glucose weekly up to 30 weeks of age. The percentage incidence of diabetes is shown in each of the five groups at week 16, 20 and 26 of age.

As can be seen in FIG. 9, soluble Ig-INSβ delayed the onset of diabetes and no animals had hyperglycemia by week 16 of age. Such delay persisted until week 20 but most of the mice developed diabetes by week 26. No such delay was observed with soluble Ig-HEL indicating that the effect on diabetes by Ig-INSβ is antigen specific. Surprisingly, however, agg Ig-INSβ delayed diabetes in all mice except 1 up to week 20 and such delay remained significant by week 26 where only 30 percent of the mice had high blood glucose while 80% of the untreated mice became diabetic (FIG. 9 b). It is worth noting that Ig-HEL which induces IL-10 production by APCs displayed significant delay of diabetes up to week 20 possibly due to IL-10 bystander suppression (FIG. 9 b).

These results indicate that agg Ig-INSβ is effective in delaying the onset of diabetes when administered at the pre-insulitis stage and suggest that IL-10 displays a down-regulatory function at this stage.

Example 10 Administration of agg Ig-INSβ into IL-10^(−/−) NOD Mice at the Pre-Insulitis Stage Does Not Delay Onset of Diabetes

The role of agg Ig-INSβ-induced IL-10 on the suppression of diabetes became evident when IL-10^(−/−) mice did not delay their diabetes onset upon treatment with agg Ig-INSβ while IL-10^(+/+) did. Groups (10 mice per group) of female wild type (IL-10^(+/+)) and IL-10^(−/−) NOD mice were given i.p. 300 μg of agg Ig-INSβ on week 4, 5 and 6 of age and monitored for blood glucose weekly. Shown is the percentage incidence of diabetes in both IL-10^(−/−) and IL-10^(+/+) mice at week 12, 16 and 20 of age after receiving the injections of agg Ig-INSβ. The results emphasize the importance of IL-10 on the suppression of diabetes in the preinsultits stage (see FIG. 10).

Example 11 Splenic and Islet Diabetogenic T Cells Develop Opposite Responses Against agg Ig-INSβ

In 4 week old mice, islet infiltration has not taken place and most of the diabetogenic T cells remain peripheral while in IAA-positive mice, which would have reached the age of 14 weeks by completion of treatment with Ig-INSβ, insulitis would be advanced and most of the diabetogenic T cells would have infiltrated the islets,(4). Thus, the difference in the delay of diabetes by agg Ig-INSβ in young versus IAA-positive mice may be due to a variable susceptibility to IL-10 of islet versus peripheral T cells.

To test this premise, splenic and islet cells from 14 week old mice were stimulated with agg Ig-INSβ, which induces IL-10 production by the presenting APCs and secretion of IFNγ was measured. Splenic (a) and islet (b) cells (5×10⁵ cells/well) from 14 week old female NOD mice were stimulated with the indicated antigen in the presence or absence of 1 ng of rIL-10 for 24 hours. The supernatant (100 μl/well) was used to measure IFNγ by ELISA as indicated in “Materials and Methods”. INSβ peptide was used at 18 μM and agg and soluble Ig-INSβ chimeras were used at 1 μM concentration. Each bar represents the mean+SD of triplicate wells for splenocytes and duplicate wells for islet cells.

As can be seen in FIG. 11, both splenic and islet T cells developed IFNγ responses upon stimulation with INSβ or soluble Ig-INSβ. However, stimulation with agg Ig-INSβ reduced IFNγ response by splenic T cells but enhanced the islet T cell response significantly. Similar effects were observed when the cells were stimulated with soluble Ig-INSβ or INSβ peptide in the presence of IL-10. These results indicate that islet and peripheral INSβ-specific T cells display differential susceptibility to IL-10.

Example 12 Sustained Administration of Soluble Ig-INSβ to Female NOD Mice after IAA Seroconversion Delays Onset of Diabetes

A study was performed to assess the impact of sustained administration of soluble Ig-INSβ or Ig-HEL to female NOD mice that had previously undergone IAA seroconversion. Groups (n=10) of female NOD mice between the ages of 7 and 11 and positive for IAA were given a weekly interperitoneal injection of 300 μg of soluble Ig-INSβ or Ig-HEL beginning on the week of seroconversion and continuing until week 12 post-seroconversion. For mice that seroconverted on week 7, each mouse received an injection on weeks 7, 8, 9, 10, 11, and 12, and biweekly thereafter; for mice that seroconverted on week 8, each mouse received an injection on weeks 8, 9, 10, 11, and 12, and biweekly thereafter; for mice that seroconverted on week 9, each mouse received an injection on weeks 9, 10, 11, and 12, and biweekly thereafter; for mice that seroconverted on week 10, each mouse received an injection on weeks 10, 11, and 12, and biweekly thereafter; and for mice that seroconverted on week 11, each mouse received an injection on weeks 11 and 12, and biweekly thereafter. Subsequent to week 12 post-seroconversion, each mouse received an injection of 300 μg of soluble Ig-INSβ or Ig-HEL every 2 weeks until the mouse reached the age of 30 weeks. A third, control group received no injections throughout the duration of the study.

Results of the study, shown in FIG. 12, indicate that sustained treatment, as described above, with sol Ig-INSβ (black bars), when administered after IAA seroconversion, significantly suppresses, delays and/or prevents the onset of diabetes by comparison with control (open bars) or Ig-HEL (hatched bars). While well over 80% of the untreated female NOD mice developed diabetes by week 30, only 3 out of 10 mice treated repeatedly with soluble Ig-INSβ developed diabetes. Mice treated with control sol Ig-HEL were not significantly protected against diabetes.

Example 13 Administration of Soluble Ig-GAD2 at the Pre-Diabetic Stage

NOD mice were assessed for blood glucose beginning at week 12 of age. Those mice that reached glucose levels of 160-250 mg/dl between week 14 to 25 received the following Ig-GAD2 regimen: The mice were given 500 μg of soluble Ig-GAD2 i.p. daily for 5 days and then weekly injections thereafter for either 15 or 25 weeks. Blood glucose monitoring was performed during this period. Results are shown in FIG. 13. Overall, 100% of mice that became pre-diabetic at the age of 14-25 weeks and that were not treated with Ig-GAD2 progressed to diabetes (blood sugar level 300 mg/dl glucose) within 5 weeks after diagnosis of the pre-diabetic stage. Moreover, 60% of mice undergoing the 15-week treatment regimen were protected against diabetes throughout the 25 week post-hyperglycemia monitoring period. Interestingly, one mouse (FIG. 13 B, left panel, open stars) progressed to diabetes by 5 weeks of treatment and 3 mice (FIG. 13 B, plus, open diamond, and open pentagon) had similar disease manifestations shortly after interruption of the treatment. When the regimen was extended to 25 weeks, 100% of the Ig-GAD2 treated animals were protected (FIG. 13 A, right panel) and normoglycemia was restored in all mice (FIG. 13 B, right panel). This status persisted throughout the duration of the study, which was terminated when the mice were 52 to 56 weeks of age.

Blood glucose levels for sol Ig-GAD2 (through week 24 of treatment) treated mice are shown in Table 1, below. TABLE 1 Blood Glucose Levels (mg/dl) for Treated Mice Mouse Week 1 2 3 4 5 6 7 8 9 10 11 12 13 14 0 161 165 180 182 165 250 179 212 160 229 232 224 180 173 1 252 125 134 159 144 137 129 179 152 258 183 154 165 199 2 176 119 213 127 144 136 169 165 146 162 227 192 152 148 3 121 117 145 121 117 255 142 228 281 285 217 186 112 111 4 149 110 127 148 126 179 124 151 390 176 214 156 159 132 5 131 144 175 117 116 153 126 128 351 98 99 161 140 136 6 148 132 114 136 150 126 123 143 94 134 97 118 156 7 98 99 146 133 93 105 121 156 89 120 179 135 134 8 128 111 178 152 113 158 119 139 170 127 172 134 108 9 109 104 140 110 120 138 153 147 147 134 142 116 132 10 118 108 160 138 120 140 121 141 145 170 132 117 151 11 151 91 192 144 101 145 113 152 143 112 114 135 163 12 107 91 244 161 130 151 109 216 150 124 149 121 97 13 107 101 256 124 113 137 108 184 142 114 130 148 137 14 85 81 264 125 116 112 119 155 154 127 154 118 143 15 133 113 198 96 120 118 99 156 147 119 178 123 158 16 136 91 285 112 128 103 112 127 153 144 146 157 17 111 129 377 105 111 148 107 134 228 123 123 111 18 127 99 366 98 158 113 148 350 159 122 93 19 99 110 111 176 137 338 339 170 132 20 94 82 119 152 130 229 256 172 21 83 96 114 135 153 331 215 22 75 101 140 133 440 23 70 99 140 154 24 90 100 150 118

Blood glucose levels for the untreated mice are shown in Table 2, below. TABLE 2 Blood Glucose Levels (mg/dl) for Untreated Mice Mouse Week 11 12 13 14 15 16 17 0 174 169 169 168 175 199 219 1 293 366 155 159 251 240 379 2 352 400 157 200 340 450 400 3 457 — 200 249 450 — — 4 — — 270 393 — — — 5 — — 376 400 — — — 6 — — 400 — — — —

Example 14

Detailed histopathologic analysis from mice in Example 13 was performed. While most of the islets in hyperglycemic and diabetic mice exhibited intra-insulitis (FIG. 14, panels 1, 2 and 3), the majority of islets in treated mice were not inflamed (FIG. 14, panel 4) or had only mild peri-insulitis (FIG. 14, panels 5 and 6). Overall, the histopathologic analysis indicated that treated mice had a significant number of islets with mild or no infiltration when compared to both hyperglycemic and diabetic mice (FIG. 14). Moreover, enumeration of islets with 20% or more non-infiltrated tissue indicated that the treatment with Ig-GAD2 led to an increase in the total number of islets relative to the hyperglycemic mice (FIG. 15). This suggests that the treated mice have more islets than they started with at the hyperglycemic stage. Analysis of islet infiltration scores among the different groups of mice indicated that the 15-week group had a higher number of islets with periinsulitis (38% vs. 30%) or no insulitis (35% vs. 17%) relative to the hyperglycemic stage (FIG. 16). On the other hand, the number of islets with severe- and mild-intrainsulitis were reduced in the treated versus hyperglycemic mice (8% and 19% vs. 22% and 31%, respectively) (FIG. 16). Surprisingly, in the 25-week treatment group, although the total number of islets was reduced to that of the hyperglycemic stage, most of these islets exhibited no (60%), peri-(28%) or mild intra- (12%) insulitis (FIG. 16). Overall, the treatment with Ig-GAD2 led to a significant increase in the number of noninflammed (“healthy”) islets that restored and maintained normoglycemia.

Example 15

An experiment was conducted to determine whether the healthy islets discussed in Example 14 were a result of a regression of inflammation and/or regeneration of beta cells. To address this question, the treated mice from Example 14 were injected with the proliferation indicator 5-bromo-2-deoxyuridine (BrdU), sacrificed and pancreatic sections were stained with anti-insulin and anti-BrdU antibodies and analyzed for BrdU incorporation and insulin production. BrdU staining was visible in the highly proliferative luminal intestinal cells but these had no staining with anti-insulin antibody (FIG. 17). Islets of non-diabetic 5-week old NOD mice were positive when stained with anti-insulin antibody, but did not incorporate BrdU, suggesting that these insulin-producing beta cells were not newly generated cells (FIG. 18). Thus, under normal circumstances insulin production emanates from existing beta cells whose nuclei do not incorporate BrdU giving a minimal number of BrdU/insulin double-positive (BrdU⁺/insulin⁺) beta cells (FIG. 19). Sections from hyperglycemic mice showed very few insulin-producing beta cells and no BrdU incorporation (FIG. 20) resulting in an insignificant number of BrdU⁺/insulin⁺ beta cells (FIG. 19). In contrast, islets from the 25-week treatment group showed beta cells that stained positive for insulin and were either BrdU negative (previously generated beta cells) or BrdU positive (newly generated beta cells) (FIG. 21). Notably, the number of these insulin-producing regenerating beta cells was significantly increased in all five mice in which treatment restored normoglycemia (FIG. 19). Interestingly the total number of regenerating cells producing insulin (Insulin+/BrdU⁺) was low and may not solely account for the restoration of normoglycemia. Insulin-positive/BrdU-negative islet cells may have also contributed to the control of blood glucose level and these likely represent a combination of newly regenerated and previously existing beta cells. There were also numerous BrdU positive/insulin-negative islet cells that likely represent newly regenerating cells that are not yet producing abundant insulin (FIG. 21). Collectively these findings suggest that this antigen-specific immunomodulation allows for islet regeneration and may be the most effective compensatory mechanism that can overcome progressive beta cell destruction. The fact that these mice were not infused with precursors of beta cells such as stem cells make these findings all the more significant. Moreover, despite that the treatment involved a single epitope, it led to islet regeneration.

U.S. patent application Ser. No. 08/779,767, filed Jan. 7, 1997, U.S. patent application Ser. No. 10/277,264, filed Oct. 21, 2002, U.S. patent application Ser. No. 09/111,123 filed Jan. 7, 1998, U.S. patent application Ser. No. 09/623,728 filed Sep. 5, 2000, U.S. patent application Ser. No. 08/873,901 filed Jun. 4, 2001 are all hereby incorporated by reference in their entireties.

For all formulations herein, multiple doses may be proportionally compounded as is known in the art. The invention has been described in an illustrative manner, and it is to be understood the terminology used is intended to be in the nature of description rather than of limitation. Many modifications, equivalents, and variations of the present invention are possible in light of the above teachings, therefore, it is to be understood that within the scope of the appended claims, the invention may be practiced other than as specifically described.

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1. A method of reversing type 1 diabetes in a subject in need thereof, the method comprising: (a) diagnosing the subject as having diabetes, and (b) administering to the subject a pharmaceutically acceptable composition comprising at least one immunoglobulin selected from the group consisting of INS, GAD, an insulin protein, a peptide derived from insulin, a diabetogenic epitope, and a T cell receptor engaging determinant; wherein the composition is administered to the subject in one or more dosage administrations.
 2. The method, of claim 1, wherein the immunoglobulin is human or humanized.
 3. The method of claim 1, wherein the subject is a human subject.
 4. The method of claim 1, wherein administration of the composition to the subject results in down regulation of an autoreactive T cell.
 5. The method of claim 1, wherein a peptide is inserted within at least one variable region of the immunoglobulin.
 6. The method of claim 5, wherein the at least one variable region of the immunoglobulin comprises a CDR1, a CDR2, and/or a CDR3 region.
 7. The method of claim 5, wherein activation of an autoreactive T cell specific for the peptide is substantially reduced or prevented.
 8. The method of claim 1, wherein the INS comprises INSβ.
 9. The method of claim 8, wherein the INSβ is soluble.
 10. The method of claim 9, wherein the soluble INSβ is capable of binding to at least one Fc receptor.
 11. The method of claim 10, wherein the Fc receptor is a Fcγ receptor.
 12. The method of claim 10, wherein the composition is endocytosed by antigen presenting cells.
 13. The method of claim 1, wherein the GAD comprises GAD 1, GAD2, or GAD65.
 14. The method of claim 13, wherein the GAD is solubilized.
 15. The method of claim 1, wherein the subject is GAD positive.
 16. The method of claim 1, wherein upon administration of the composition to the subject, the subject undergoes restoration of normoglycemia.
 17. The method of claim 16 wherein the subject undergoes restoration of normoglycemia without assistance of exogenous insulin or stem cell infusion. 